AU2006288279A1 - Promoter for introducing gene into lymphocyte or blood cell and application thereof - Google Patents

Description

VERIFICATION OF TRANSLATION International Patent Application No. PCT/JP2006/317574 by The Research Foundation for Microbial Diseases of Osaka University I, MqsOori MATS (AO of 41-m-~2. iamvack'i, Ckvoiz Al Osaka-sklf Oso -f S/+0--003 Tapcw\ am the translator of the documents attached and I state that the following is a true translation to the best of my knowledge and belief of International Patent Application No. PCT/JP20061317574 dated 5 September 2006. DATED this f - day of Mf 6rd , 2008 (Signature of translator) -1 - OBK008 DESCRIPTION PROMOTER FOR INTRODUCING A GENE INTO A LYMPHOCYTE OR BLOOD CELL AND APPLICATION THEREOF 5 TECHNICAL FIELD (0001] The present invention is related to a promoter for 10 introducing a gene into lymphocytes or blood cells, and the application thereof. BACKGROUND ART 15 [0002] There has been a demand for the establishment of a technique for gene therapy on lymphoid cells in order to treat various diseases targeting lymphoid cells, e.g., human immunodeficiency virus (HIV) infection. However, no 20 satisfactory vector system for introducing a desired gene into lymphoid cells has been developed. [0003] Herpesvirus (HHV) is a generic term referring to viruses of the family Herpesviridae. Both human 25 herpesvirus 6 and 7 (HHV-6 and HHV-7) are double-stranded DNA viruses of the subfamily P Herpesviridae of the family Herpesviridae, which are responsible for exanthem subitum. (Yamanishi K. et al., "Identification of human herpesvirus 6 as a casual agent for exanthem subitum", Lancet 1988; i: 30 1065-1067 and Tanaka K. et al., "Human herupesvirus 7: Another casual agent for roseola (exanthem subitum)", J. pediatr., 1994; 125: 1-5) HHV-6 includes two strains, HHV- -2- OBKO08 6A and HHV-6B. HHV-6 causes a viral infectious disease which'often occurs during infancy and induces sudden high fever and exanthema before and after the reduction of fever. Its prognosis is generally good. HHV-7 infection tends to 5 occur later than HHV-6 infection (Tanaka K. et al., "Seroepidemiological study of human herpesvirus-6 and -7 in children of different ages and detection of those two viruses in throat swabs by polymerase chain reaction", Journal of Medical Virology, 1996; 48: 88-94). Therefore, 10 exanthem subitum caused by HHV-7 is clinically experienced as second exanthem subitum. A seroepidemiological study of HHV-6 and HHV-7 demonstrated that most children become positive for antibodies for HHV-6 and HHV-7 before the age of two or three. It has been reported that the inapparent 15 infection rate is 20 to 40%. [0004] HHV-7 is a herpesvirus which was newly found by Frenkel et al. in 1990 when a cytopathic effect occurred during culturing of CD4* T lymphoid cells of a healthy 20 person's peripheral blood (Frankel N. et al., "Isolation of a new herpesvirus from human CD4C T cells", ProNAS USA, 87: 749-752, ProNAS USA, 87: 749-752, 1990). The virus was isolated from mononuclear cells of human peripheral blood. Both HHV-6 and -7 are CD4' T lymphoid cell tropic viruses. 25 HHV-7 infects the cell via a CD4 receptor on the cell. HHV-7 can grow only in human T lymphoid cells. Therefore, HHV-7 is a virus which can be used for gene modification of human T lymphoid cells. [0005] 30 The HHV-7 genome is double-stranded DNA of about 145 kbp. The whole base sequence has been determined by Nicholas et al. It is known that at least 101 genes are -3- OBKO08 present on the genome (John N. et al., Journal of Virology, Sep. 1996, 5975 to 5989). [0006] However, with respect to these HHVs, no detailed 5 analysis has been conducted so far regarding the promoter activity thereof. Moreover, what is lymphoid cell specific for the viruses was due to the interaction with receptors in the cells, and the life cycle in which the viruses can only be propagated in a human T-lymphocytes. 10 [00071 In addition, it is believed that these viruses, particularly HHV-7 virus, have no adverse effect on healthy persons. If a gene containing an antigenic determinant of various viruses (e.g., mumps) is incorporated into the 15 viral genome of HHV-7 and is expressed in HHV-7, HHV-7 is considered to be useful as a vaccine. However, when HHV-7 is used as a vaccine, it is not preferable that the genotype is changed as the virus is subcultured, in terms of quality control and quality assurance. Therefore, when 20 the recombinant virus is used as a vaccine, it is necessary to stably supply a virus derived from a single recombinant genotype virus. For this purpose, a technique for producing a HHV-7 recombinant virus having a single genotype has been desired. 25 [0008] In addition, the mutual relationship between the HIV infection of a T lymphoid cell strain SupT1 cell and a T lymphoid cell tropic human herpesvirus (HHV-6A (U1102 strain), HHV-7 (MRK, MSO strains)) has been studied. 30 The HHV-7 strain, which is bound by a CD4 receptor of cells, exhibits satisfactory growth in SupT1 cells. However, infection could not been established for SupTl/HIV cells.

-4- OBKO08 In contrast, it has been recognized that the HHV-6A strain infects HIV-persistent infection SupT1 (SupTl /HIV) cells and exhibits clear CPE (Masao Yamada et al., "HIV Jizokukansen SupT1 Saibo heno HHV-6 oyobi -7 5 Choufukukannsen no Kokoromi (Attempt for HHV-6 and -7 Superinfection to HIV Persistent Infection Sup-Tl Cell)", Title No. 122, Titles and Abstracts of the 7th Annual Meeting of the Japanese Society for AIDS Research, 1993, Tokyo). 10 [00091 An ideal HIV vaccine can provide perfect and long-term protection from all types of HIV. On the other hand, conventional inactivated HIV vaccines have advantages and disadvantages, some of which will be described below. 15 A method for producing a recombinant vaccine employs common techniques. However, since it is difficult to maintain immunogenicity (since immunogenicity is low), high antigenic load and frequent inoculation of an adjuvant are required. Safety is the greatest concern. A subunit 20 vaccine containing either a native or recombinant subunit may be safe. However, such a subunit vaccine requires high antigen load and frequent vaccination with adjuvant, because of the use of a subunit and the low immunogenicity. Moreover, safety is the most important issue. Furthermore, 25 subunit vaccines comprising either a native or a recombinant subunit may be safe, however, they are subjected to limitation due to low selectivity and low immunogenicity of the subunit, thereby they allow development of usable vaccines for treating an immune 30 responsible cell such as HIV vaccines and the like.

-5- OBK008 [non-patent literature 1]Yamanishi K et al., "Identification of human herpesvirus 6 as a casual agent for exanthem subitum."Lancet 1988;i: pp. 1065-1067 [non-patent literature 2]Tanaka K et al., "Human 5 herpesvirus 7: Another casual agent for roseola (exanthem subitum)"J pediatr.1994;125:pp.1-5 [non-patent literature 3]Tanaka-Taya K et al.,"Seroepidemiological study of human herpesvirus-6 and 7 in children of different ages and detection of those two 10 viruses in throat swabs by polymerase chain reaction" Journal of Medical Virology. 1996;48: pp.88-94 [non-patent literature 4] Frankel N et al.,,"Isolation of a new herpesvirus from human CD4+T cells. "ProNAS USA 87:749 15 752,ProNAS USA 87:749-752,1990 [non-patent literature 5]John N. et al.,,Journal of Virology, Sep.1996, pp. 5975-5989 [non-patent literature6] Masao Yamada et al., "HIV Jizokukansen SupT1 Saibo heno HHV-6 oyobi -7 20 Choufukukannsen no Kokoromi (Attempt for HHV-6 and -7 Superinfection to HIV Persistent Infection Sup-T1 Cell)", Title No. 122, Titles and Abstracts of the 7th Annual Meeting of the Japanese Society for AIDS Research, 1993, Tokyo 25 DISCLOSURE OF THE INVENTION PROBLEM TO BE SOLVED BY THE INVENTION 30 [0010] It is an object of the present invention to provide a promoter which induces gene expression in an immune system -6- OBKO08 cell or blood cell such as lymphoid cells, in a selective and potent manner. MEANS FOR SOLVING THE PROBLEM 5 [0011] The above mentioned problems have been solved by the present invention by discovering that MIE promoter of HHV6, MIE promoter of HHV67,m and U95 promoter of HHV7 10 surprisingly induce specific expression in an immune responsible cell such as T lymphoid cell, or hemocyto lineage cells. [0012] In development of DNA vaccines, which are an 15 attractive new technology, potent expression promoters are essential. To date, human cytomegalovirus (HCMV) immediate early (IE) promoter is widely used in DNA vaccines. This is due to the fact that HCMV IE promoters are believed to exhibit potent activity in a variety of cells in general. 20 However, it is reported that the expression efficiency thereof is low in lymphoid lineage cells, and the phenomenon of inactivation due to methylation and the like is observed. Moreover, there are problems associated with a variety of restrictions which inhibit realization of the 25 application of the HHV IE promoter on DNA vaccines. [0013] HCMV is known to have a limited number of cells which it can infect, but is known to infect fibroblast cells and blood endothelial cells and the like. On the other hand, 30 HHV-6 infects human infants and causes exanthema subitum or roseola infantum, and it is known that it proliferates well in human lymphocytes, in particular, T cells. The present -7- OBKO08 inventors have elucidated in the present invention that major immediate early gene '(MIE) of HHV-6, which belongs to the same 8 virus subgenus of the human herpesvirus genus, the same as HCMV, exhibits strong promoter activity. The 5 present inventors have also elucidated that the MIE gene promoter is available for DNA vaccines. HHV-7 is also a CD4* T lymphocyte directed virus, and the promoter thereof can be used to develop DNA vaccines, for example, to prevent or treat a disease related to CD4C T lymphocytes. 10 The present inventors have elucidated in the present invention the utility of HHV 7 MIE promoter and HHV 7 U95 promoter, and thus also elucidated that these promoters can be used for DNA vaccines. [0014] 15 Therefore, the present invention provides the following: [0015] (1) An MIE promoter of HHV6B. [00161 20 (2) The promoter according to item 1, which comprises at least eight contiguous nucleotides of the sequence set forth in SEQ ID NO: 1. [0017] (3) The promoter according to item 1, which comprises 25 at least the R3 region of the sequence set forth in SEQ ID NO: 1 or a functional variant thereof. [0018] (4) The promoter according to item 1, which comprises at least the sequence of -574 to -427 (SEQ ID NO: 13) from 30 the transcription initiation point of the SEQ ID NO: 1. [0019] -8- OBKO08 (5) The promoter according to item 1, which comprises at least the sequence of -1051 to -427 (SEQ ID NO: 14) from the transcription initiation point of SEQ ID NO: 1. [0020] 5 (6) The promoter according to item 1, which comprises a motif of NF-KB and a motif of AP-1. [0021] (7) The promoter according to item 1, which comprises the sequence set forth in SEQ ID NO: 1. 10 [0022] (8) The promoter according to item 1, wherein the promoter comprises: (a) a polynucleotide having the base sequence set forth in SEQ ID NO: 1, or the base sequence corresponding thereto or a fragment sequence thereof; 15 (b) a polynucleotide of an allelic variant of the base sequence set forth in SEQ ID NO: 1 or the base sequence corresponding thereto or a fragment sequence thereof; (c) a polynucleotide which hybridizes a polynucleotide of any of (a) or (b) and has a biological activity thereof; or 20 (d) a polynucleotide which consists of the base sequence of any of (a) to (c) or a complement sequence thereof with at least 70 % identity, and has a biological activity thereof. [0023] (9) The promoter according to item 1, which is at least 10 25 contiguous nucleotides in length. [0024] (10) The promoter according to item 8, wherein the biological activity is the promoter activity. [00251 30 (11) A nucleic acid construct comprising the promoter according to item 1. [0026] -9- OBKO08 (12) The nucleic acid construct according to Item 11, which comprises a sequence encoding a foreign gene which is not related to the promoter but is operatively linked to the sequence of the promoter. 5 [0027] (13) The nucleic acid construct according to item 12, wherein the foreign gene encodes an RNAi molecule, a drug, a recessive gene to be deleted, or a selective marker. [0028] 10 (14) The nucleic acid construct according to item 13, wherein the selective marker allows selection in a medium of a host in which the nucleic acid construct is introduced. [0029] (15) The nucleic acid construct according to item 13, 15 wherein the selective marker allows visual selection in a host in which the nucleic acid construct is introduced. [0030] (16) The nucleic acid construct according to item 13, wherein the selective marker comprises hypoxanthine guanine 20 phosphoribosyl transferase (hprt) or a fluorescent marker selected from the group consisting of green fluorescent protein (GFP), cyan fluorescent protein (CFP), yellow fluorescent protein (YFP) and red fluorescent protein (dsRed). 25 [0031] (17) The nucleic acid construct according to item 13, wherein the selective marker does not substantially exhibit toxicity against the host in which the nucleic acid construct is introduced. 30 [0032] (18) The nucleic acid construct according to item 13, wherein the recessive gene to be deleted is selected from -10- OBK008 the group consisting of ADA gene, PNP gene, y c chain gene, TAP gene, MHC II gene, X-linked WASP, CD40 ligand, P13K like gene and DNA helicase. [0033] 5 (19) The nucleic acid construct according to item 13, wherein the drug is selected from the group consisting of a cytokine, a chemokine, a growth factor, a protein hormone, and a peptide hormone (e.g. interferon (IFN)-a, IFN-y, interleukin [IL]-2, IL-12, granulocyte colony stimulating 10 factor [G-CSF], granulocyte macrophage colony stimulating factor [GM-CSF]). [0034] (20) The nucleic acid construct according to item 12, wherein the promoter induces specific expression of the 15 foreign gene in a hemocyto-lineage cell, in particular, in a T cell. [0035] (21) An expression vector comprising the nucleic acid construct according to item 11. 20 [0036] (22) A cell comprising the nucleic acid construct according to item 11. [0037] (23) The cell according to item 22, wherein the cell is 25 heterogenous to the promoter sequence. [00381 (24) A tissue comprising the nucleic acid construct according to item 11. [00391 30 (25) An organ comprising the nucleic acid construct according to item 11. [00401 -11- OBKO08 (26) An organism comprising the nucleic acid construct according to item 11. [0041] (27) A pharmaceutical composition comprising the promoter 5 according to item 1 and a sequence encoding an antigen. [0042] (28) The pharmaceutical composition according to item 27, which is a DNA vaccine. [0043] 10 (29) A pharmaceutical composition for treating a disease, disorder or condition in which a lymphocyte-specific treatment is desired, which comprises the promoter according to item 1, and a nucleic acid sequence for the treatment. 15 [0044] (30) The pharmaceutical composition according to item 29, wherein the nucleic acid sequence for the treatment comprises a sequence selected from the group consisting of those encoding cytokines, chemokines, growth factors, 20 protein hormones, peptide hormones, ribozymes and RNAis (HIV-1 gp4l: AATAAGACAGGGCTTGGAAAGACACTTTCCAAGCCCTGTCTTATTTTT ( SEQ ID NO: 33)/HIV-1 tat: AAGCATCCAGGAAGTCAGCCTACAAGGCTGACTTCCTGGATGCTTTTT(SEQ ID NO: 25 34)/HTLV-1 tax: GAACATTGGTGAGGAAGGCACAGCCTTCCTCACCAATGTTCTTTTT(SEQ ID NO: 35)). [0045] (31) A method for expressing a protein in a lymphocyte 30 specific manner, comprising the steps of: -12- OBKO08 A) preparing a nucleic acid construct in which the promoter according to item 1 is operatively linked to a nucleic acid sequence encoding the protein; and B) placing the nucleic acid construct under a 5 condition in which the promoter induces the expression of the nucleic acid sequence encoding the protein. [0046] (32) A kit for expressing a protein in a lymphocyte specific manner, comprising: 10 A) a nucleic acid construct in which the promoter according to item 1 is operatively linked to a nucleic acid sequence encoding the protein; and B) means for placing the nucleic acid construct under a condition in which the promoter induces the expression of 15 the nucleic acid sequence encoding the protein. [0047] (33) A kit for expressing a protein in a lymphocyte specific manner, comprising: A) the promoter according to item 1; and 20 B) means for producing a nucleic acid construct in which the promoter is linked to a nucleic acid sequence encoding the protein. [0048] (34) A method for treating or preventing a disease, 25 disorder or condition which requires the expression of a protein in a lymphocyte specific manner, comprising the steps of: A) producing a nucleic acid construct in which the promoter according to item 1 is linked to a nucleic acid 30 sequence encoding the protein; and -13- OBKO08 B) placing the nucleic acid construct under a condition in which the promoter induces the expression of the nucleic acid sequence encoding the protein. [0049] 5 (35) A kit for treating or preventing a disease, disorder or condition which requires the expression of a protein in a lymphocyte specific manner, comprising: A) a nucleic acid construct in which the promoter according to item 1 is linked to a nucleic acid sequence 10 encoding the protein; and B) means for placing the nucleic acid construct under a condition in which the promoter induces the expression of the nucleic acid sequence encoding the protein. [0050] 15 (36) A kit for treating or preventing a disease, disorder or condition which requires the expression of a protein in a lymphocyte specific manner, comprising: A) the promoter according to item 1; and B) means for producing a nucleic acid construct in 20 which the promoter is linked to a nucleic acid sequence encoding the protein. [0051] (37) A method for producing a protein, comprising the steps of: 25 A) preparing a nucleic acid construct in which the promoter according to item 1 is linked to a nucleic acid sequence encoding the protein; and B) placing the nucleic acid construct under a condition in which the promoter induces the expression of 30 the nucleic acid sequence encoding the protein. [0052] (38) A kit for producing a protein, comprising: -14- OBKO08 A) a nucleic acid construct in which the promoter according to item 1 is linked to a nucleic acid sequence encoding the protein; and B) means for placing the nucleic acid construct under 5 a condition in which the promoter induces the expression of the nucleic acid sequence encoding the protein. [0053] (39) A kit for producing a protein, comprising: A) the promoter according to item 1; and 10 B) means for producing a nucleic acid construct in which the promoter is linked to a nucleic acid sequence encoding the protein. [0054] (40) Use of the promoter according to item 1, for 15 manufacture of a pharmaceutical composition for treating or preventing a disease, disorder or condition which requires the expression of a protein in a lymphocyte specific manner. [0055] (41) An MIE promoter of HHV7. 20 [0056] (42) The promoter according to item 41, which comprises at least eight contiguous nucleotides of the sequence set forth in SEQ ID NO: 2. [0057] 25 (43) The promoter according to item 41, which comprises at least the R2 region of the sequence set forth in SEQ ID NO: 2 or a functional variant thereof. [00581 (44) The promoter according to item 41, which comprises at 30 least the sequence of +22 to -233 of the SEQ ID NO: 2. [0059] -15 - OBKO08 (45) The promoter according to item 41, which comprises at least the sequence of +22 to -388 of the SEQ ID NO: 2. [0060] (46) The promoter according to item 41, which comprises a 5 motif of NF-KB present in the R2 region. [0061] (47) The promoter according to item 41, which comprises the sequence set forth in SEQ ID NO: 15. [0062] 10 (48) The promoter according to item 41, wherein the promoter comprises: (a) a polynucleotide having the base sequence set forth in SEQ ID NO. 2, or a base sequence corresponding thereto or a fragment sequence thereof; 15 (b) a polynucleotide of an allelic variant of the base sequence set forth in SEQ ID NO. 2 or the base sequence corresponding thereto or a fragment sequence thereof; (c) a polynucleotide which hybridizes a polynucleotide of any of (a) or (b) and has a biological activity thereof; or 20 (d) a polynucleotide which consists of the base sequence of any of (a) to (c) or a complement sequence thereof with at least 70 % identity, and has a biological activity thereof. [0063] (49) The promoter according to item 41, which is at least 25 10 contiguous nucleotides in length. [0064] (50) The promoter according to item 48, wherein the biological activity is the promoter activity. [0065] 30 (51) A nucleic acid construct comprising the promoter according to item 41. [0066] -16- OBKO08 (52) The nucleic acid construct according to Item 51, which comprises a sequence encoding a foreign gene which is not related to the promoter but is operatively linked to the sequence of the promoter. 5 [0067] (53) The nucleic acid construct according to item 52, wherein the foreign gene encodes an RNAi molecule, a drug, a recessive gene to be deleted, or a selective marker. [0068] 10 (54) The nucleic acid construct according to item 53, wherein the selective marker allows selection in a medium of a host in which the nucleic acid construct is introduced. [0069] (55) The nucleic acid construct according to item 53, 15 wherein the selective marker allows visual selection in a host in which the nucleic acid construct is introduced. [0070] (56) The nucleic acid construct according to item 53, wherein the selective marker comprises hypoxanthine guanine 20 phosphoribosyl transferase (hprt) or a fluorescent marker selected from the group consisting of green fluorescent protein (GFP), cyan fluorescent protein (CFP), yellow fluorescent protein (YFP) and red fluorescent protein (dsRed). 25 [0071] (57) The nucleic acid construct according to item 53, wherein the selective marker does not substantially exhibit toxicity against the host in which the nucleic acid construct is introduced. 30 [0072] (58) The nucleic acid construct according to item 53, wherein the recessive gene to be deleted is selected from -17- OBKO08 the group consisting of ADA gene, PNP gene, y c chain gene, TAP gene, MHC II gene, X-linked WASP, CD40 ligand, P13K like gene and DNA helicase. [0073] 5 (59) The nucleic acid construct according to item 53, wherein the drug is selected from the group consisting of a cytokine, a chemokine, a growth factor, a protein hormone, and a peptide hormone (IFN-a, IFN-y, IL-2, IL-12, G-CSF, GM-CSF). 10 [0074] (60) The nucleic acid construct according to item 52, wherein the promoter induces specific expression of the foreign gene in a hemocyto-lineage cell, in particular, in a T cell. 15 (0075] (61) An expression vector comprising the nucleic acid construct according to item 51. [0076] (62) A cell comprising the nucleic acid construct according 20 to item 51. [0077] (63) The cell according to item 62, wherein the cell is heterogenous to the promoter sequence. [0078] 25 (64) A tissue comprising the nucleic acid construct according to item 51. [0079] (65) An organ comprising the nucleic acid construct according to item 51. 30 [0080] (66) An organism comprising the nucleic acid construct according to item 51.

-18- OBK008 [0081] (67) A pharmaceutical composition comprising the promoter according to item 41 and a sequence encoding an antigen. [0082] 5 (68) The pharmaceutical composition according to item 67, which is a DNA vaccine. [0083] (69) A pharmaceutical composition for treating a disease, disorder or condition in which a lymphocyte-specific 10 treatment is desired, which comprises the promoter according to item 41, and a nucleic acid sequence for the treatment. [0084] (70) The pharmaceutical composition according to item 69, 15 wherein the nucleic acid sequence for the treatment comprises a sequence selected from the group consisting of those encoding cytokines, chemokines, growth factors, protein hormones, peptide hormones, ribozymes and RNAis (HIV-1 gp4l: 20 AATAAGACAGGGCTTGGAAAGACACTTTCCAAGCCCTGTCTTATTTTT(SEQ ID NO: 33)/HIV-1 tat: AAGCATCCAGGAAGTCAGCCTACAAGGCTGACTTCCTGGATGCTTTTT(SEQ ID NO: 34)/HTLV-1 tax: GAACATTGGTGAGGAAGGCACAGCCTTCCTCACCAATGTTCTTTTT(SEQ ID NO: 25 35)). [0085] (71) A method for expressing a protein in a lymphocyte specific manner, comprising the steps of: A) preparing a nucleic acid construct in which the 30 promoter according to item 41 is operatively linked to a nucleic acid sequence encoding the protein; and -19- OBKO08 B) placing the nucleic acid construct under a condition in which the promoter induces the expression of the nucleic acid sequence encoding the protein. [0086] 5 (72) A kit for expressing a protein in a lymphocyte specific manner, comprising: A) a nucleic acid construct in which the promoter according to item 41 is operatively linked to a nucleic acid sequence encoding the protein; and 10 B) means for placing the nucleic acid construct under a condition in which the promoter induces the expression of the nucleic acid sequence encoding the protein. [00871 (73) A kit for expressing a protein in a lymphocyte 15 specific manner, comprising: A) the promoter according to item 41; and B) means for producing a nucleic acid construct in which the promoter is linked to a nucleic acid sequence encoding the protein. 20 [0088] (74) A method for treating or preventing a disease, disorder or condition which requires the expression of a protein in a lymphocyte specific manner, comprising the steps of: 25 A) producing a nucleic acid construct in which the promoter according to item 41 is linked to a nucleic acid sequence encoding the protein; and B) placing the nucleic acid construct under a condition in which the promoter induces the expression of 30 the nucleic acid sequence encoding the protein. (0089] -20- OBKO08 (75) A kit for treating or preventing a disease, disorder or condition which requires the expression of a protein in a lymphocyte specific manner, comprising: A) a nucleic acid construct in which the promoter 5 according to item 41 is linked to a nucleic acid sequence encoding the protein; and B) means for placing the nucleic acid construct under a condition in which the promoter induces the expression of the nucleic acid sequence encoding the protein. 10 [0090] (76) A kit for treating or preventing a disease, disorder or condition which requires the expression of a protein in a lymphocyte specific manner, comprising: A) the promoter according to item 41; and 15 B) means for producing a nucleic acid construct in which the promoter is linked to a nucleic acid sequence encoding the protein. [0091] (77) A method for producing a protein, comprising the steps 20 of: A) preparing a nucleic acid construct in which the promoter according to item 41 is linked to a nucleic acid sequence encoding the protein; and B) placing the nucleic acid construct under a 25 condition in which the promoter induces the expression of the nucleic acid sequence encoding the protein. [0092] (78) A kit for producing a protein, comprising: A) a nucleic acid construct in which the promoter 30 according to item 41 is linked to a nucleic acid sequence encoding the protein; and -21- OBKO08 B) means for placing the nucleic acid construct under a condition in which the promoter induces the expression of the nucleic acid sequence encoding the protein. [0093] 5 (79) A kit for producing a protein, comprising: A) the promoter according to item 41; and B) means for producing a nucleic acid construct in which the promoter is linked to a nucleic acid sequence encoding the protein. 10 [0094] (80) Use of the promoter according to item 41, for manufacture of a pharmaceutical composition for treating or preventing a disease, disorder or condition which requires the expression of a protein in a lymphocyte specific manner. 15 [0095] (81) A U95 promoter of HHV7. [0096] (82) The promoter according to item 81, which comprises at least eight contiguous nucleotides of the sequence set 20 forth in SEQ ID NO: 12. [0097] (83) The promoter according to item 81, which comprises at least the R2 region of the sequence set forth in SEQ ID NO: 12 or a functional variant thereof. 25 [0098] (84) The promoter according to item 81, which comprises at least the sequence of +16 to -233 of the SEQ ID NO: 12. [0099] (85) The promoter according to item 81, which comprises at 30 least the sequence of +16 to -379 of the SEQ ID NO: 12. [0100] -22 - OBKO08 (86) The promoter according to item 81, which comprises a motif of NF-KB present in the R2 region. [0101] (87) The promoter according to item 81, which comprises the 5 sequence set forth in SEQ ID NO: 16. [0102] (88) The promoter according to item 81, wherein the promoter comprises: (a) a polynucleotide having the base sequence set forth in 10 SEQ ID NO. 12, or the base sequence corresponding thereto or a fragment sequence thereof; (b) a polynucleotide of an allelic variant of the base sequence set forth in SEQ ID NO. 12 or the base sequence corresponding thereto or a fragment sequence thereof; 15 (c) a polynucleotide which hybridizes a polynucleotide of any of (a) or (b) and has a biological activity thereof; or (d) a polynucleotide which consists of the base sequence of any of (a) to (c) or a complement sequence thereof with at least 70 % identity, and has a biological activity thereof. 20 [0103] (89) The promoter according to item 81, which is at least 10 contiguous nucleotides in length. [0104] (90) The promoter according to item 88, wherein the 25 biological activity is the promoter activity. [0105] (91) A nucleic acid construct comprising the promoter according to item 81. [0106] 30 (92) The nucleic acid construct according to Item 91, which comprises a sequence encoding a foreign gene which is not -23- OBKO08 related to the promoter but is operatively linked to the sequence of the promoter. [0107] (93) The nucleic acid construct according to item 92, 5 wherein the foreign gene encodes an RNAi molecule, a drug, a recessive gene to be deleted, or a selective marker. [0108] (94) The nucleic acid construct according to item 93, wherein the selective marker allows selection in a medium 10 of a host in which the nucleic acid construct is introduced. [0109] (95) The nucleic acid construct according to item 93, wherein the selective marker allows visual selection in a host in which the nucleic acid construct is introduced. 15 [01101 (96) The nucleic acid construct according to item 93, wherein the selective marker comprises hypoxanthine guanine phosphoribosyl transferase (hprt) or a fluorescent marker selected from the group consisting of green fluorescent 20 protein (GFP), cyan fluorescent protein (CFP), yellow fluorescent protein (YFP) and red fluorescent protein (dsRed). [0111] (97) The nucleic acid construct according to item 93, 25 wherein the selective marker does not substantially exhibit toxicity against the host in which the nucleic acid construct is introduced. [0112] (98) The nucleic acid construct according to item 93, 30 wherein the recessive gene to be deleted is selected from the group consisting of ADA gene, PNP gene, y c chain gene, -24- OBKO08 TAP gene, MHC II gene, X-linked WASP, CD40 ligand, P13K like gene and DNA helicase. [01131 (99) The nucleic acid construct according to item 93, 5 wherein the drug is selected from the group consisting of a cytokine, a chemokine, a growth factor, a protein hormone, and a peptide hormone (IFN-a,IFN-y,IL-2,IL-12,G-CSF,GM-CSF). [0114] (100) The nucleic acid construct according to item 92, 10 wherein the promoter induces specific expression of the foreign gene in a hemocyto-lineage cell, in particular, in a T cell. [0115] (101) An expression vector comprising the nucleic acid 15 construct according to item 91. [0116] (102) A cell comprising the nucleic acid construct according to item 91. [0117] 20 (103) The cell according to item 102, wherein the cell is heterogenous to the promoter sequence. [0118] (104) A tissue comprising the nucleic acid construct according to item 91. 25 [0119] (105) An organ comprising the nucleic acid construct according to item 91. [0120] (106) An organism comprising the nucleic acid construct 30 according to item 91. [0121] -25- OBKO08 (107) A pharmaceutical composition comprising the promoter according to item 81 and a sequence encoding an antigen. [0122] (108) The pharmaceutical composition according to item 107, 5 which is a DNA vaccine. [01231 (109) A pharmaceutical composition for treating a disease, disorder or condition in which a lymphocyte-specific treatment is desired, which comprises the promoter 10 according to item 81, and a nucleic acid sequence for the treatment. [0124] (110) The pharmaceutical composition according to item 109, wherein the nucleic acid sequence for the treatment 15 comprises a sequence selected from the group consisting of those encoding cytokines, chemokines, growth factors, protein hormones, peptide hormones, ribozymes and RNAis (HIV-1 gp4l: AATAAGACAGGGCTTGGAAAGACACTTTCCAAGCCCTGTCTTATTTTT(SEQ ID NO: 20 33)/HIV-1 tat: AAGCATCCAGGAAGTCAGCCTACAAGGCTGACTTCCTGGATGCTTTTT(SEQ ID NO: 34)/HTLV-1 tax: GAACATTGGTGAGGAAGGCACAGCCTTCCTCACCAATGTTCTTTTT ( SEQ ID NO: 35)). 25 [0125] (111) A method for expressing a protein in a lymphocyte specific manner, comprising the steps of: A) preparing a nucleic acid construct in which the promoter according to item 81 is operatively linked to a 30 nucleic acid sequence encoding the protein; and -26- OBKO08 B) placing the nucleic acid construct under a condition in which the promoter induces the expression of the nucleic acid sequence encoding the protein. [0126] 5 (112) A kit for expressing a protein in a lymphocyte specific manner, comprising: A) a nucleic acid construct in which the promoter according to item 81 is operatively linked to a nucleic acid sequence encoding the protein; and 10 B) means for placing the nucleic acid construct under a condition in which the promoter induces the expression of the nucleic acid sequence encoding the protein. [0127] (113) A kit for expressing a protein in a lymphocyte 15 specific manner, comprising: A) the promoter according to item 81; and B) means for producing a nucleic acid construct in which the promoter is linked to a nucleic acid sequence encoding the protein. 20 [0128] (114) A method for treating or preventing a disease, disorder or condition which requires the expression of a protein in a lymphocyte specific manner, comprising the steps of: 25 A) producing a nucleic acid construct in which the promoter according to item 81 is linked to a nucleic acid sequence encoding the protein; and B) placing the nucleic acid construct under a condition in which the promoter induces the expression of 30 the nucleic acid sequence encoding the protein. [0129] -27- OBKO08 (115) A kit for treating or preventing a disease, disorder or condition which requires the expression of a protein in a lymphocyte specific manner, comprising: A) a nucleic acid construct in which the promoter 5 according to item 81 is linked to a nucleic acid sequence encoding the protein; and B) means for placing the nucleic acid construct under a condition in which the promoter induces the expression of the nucleic acid sequence encoding the protein. 10 [0130] (116) A kit for treating or preventing a disease, disorder or condition which requires the expression of a protein in a lymphocyte specific manner, comprising: A) the promoter according to item 81; and 15 B) means for producing a nucleic acid construct in which the promoter is linked to a nucleic acid sequence encoding the protein. [01311 (117) A method for producing a protein, comprising the 20 steps of: A) preparing a nucleic acid construct in which the promoter according to item 81 is linked to a nucleic acid sequence encoding the protein; and B) placing the nucleic acid construct under a 25 condition in which the promoter induces the expression of the nucleic acid sequence encoding the protein. [0132] (118) A kit for producing a protein, comprising: A) a nucleic acid construct in which the promoter 30 according to item 81 is linked to a nucleic acid sequence. encoding the protein; and -28 - OBKO08 B) means for placing the nucleic acid construct under a condition in which the promoter induces the expression of the nucleic acid sequence encoding the protein. [0133] 5 (119) A kit for producing a protein, comprising: A) the promoter according to item 81; and B) means for producing a nucleic acid construct in which the promoter is linked to a nucleic acid sequence encoding the protein. 10 [0134] (120) Use of the promoter according to item 81, for manufacture of a pharmaceutical composition for treating or preventing a disease, disorder or condition which requires the expression of a protein in a lymphocyte specific manner. 15 [0135] Hereinafter, preferable embodiments of the present invention are presented. It should be understood that those skilled in the art would appropriately practice the embodiments thereof based on the description of the 20 present invention in view of the well known and routinely used technology in the art, and the functions and effects attained by the present invention should be readily understood. 25 EFFECTS OF THE INVENTION [0136] The present invention provides promoters which selectively induce the expression of a protein in a cell of the immune system such as T lymphocytes. The promoters of 30 the present invention are used to provide a method and medicament for effectively preventing or treating immunological disease such as innate immune deficiency -29- OBKO08 syndrome and the like. The present invention also provides a technology in order to efficiently conduct gene therapy. BRIEF DESCRIPTION OF THE DRAWINGS 5 [0137] [Figure 1] Figure 1 depicts a comparison of promoter activities in adhesive cells. The x-axis aligns a variety of promoters, and the promoter activities of the Vero cell, the HEL cell, the L929 cell, the 293 cell and the 373 cell 10 are shown using Log(RLU)/B-gal with logarithmic reference. [Figure 2] Figure 2 depicts the comparison of promoter activities in lymphocytes. The x-axis aligns a variety of promoters, and the promoter activities of the THP-1 cell, the SupT1 cell and the U937 cell are shown using 15 Log(RLU)/B-gal with logarithmic reference. [Figure 3] Figure 3 depicts the promoter activity of the HHV-6 MIE region in the case of stimulating a cell with TPA (Vero cell). On the x-axis, a variety of promoters are aligned, and the activity of a promoter with and without 20 TPA is shown using Log(RLU)/B-gal in a logarithmic manner. [Figure 4] Figure 4 depicts promoter activity of the HHV 6 MIE region (L929 cell) when the cell has been stimulated with TPO. On the x-axis, a variety of promoters are aligned, and the promoter activity in the presence or 25 absence of TPA with respect to the respective promoters is depicted using Log(RLU)/B-gal in a logarithmic manner. [Figure 5] Figure 5 depicts illustrations of a variety of deletion variants in a promoter region of the HHV6B. The upper panel shows the promoter region, and a variety of 30 motifs in the promoter regions. [Figure 6] Figure 6 depicts a measurement system for promoter activity.

-30- OBKO08 [Figure 7) Figure 7 depicts the promoter activity (relative luciferase activity) with illustrations of a variety of deletion variants in the promoter region in the HHV6B. 5 [Figure 8] Figure 8 depicts illustrations of the immediate early (IE) gene relating to the promoter region of the HHV7 and the promoter thereof. The left column shows, from the top,7MIE promoter (-493), 7MIE promoter ( 388), and 7MIE promoter (-233), and the right column shows, 10 from the top, 7U95 promoter (-484), 7U95 promoter (-379), and 7U95promoter (-304). [Figure 9] Figure 9 depicts the activity of the IE promoter of the HHV7 in a lymphocytic cell line. The upper left graph shows Jurkat cells, the upper right graph shows 15 Molt-3 cells, the lower left graph shows SupT1 cells, and the lower right graph shows SAS-413 cells. Each graph shows, from the left, CMVP, 6MIEP, 6U95P, 7MIE(-493), 7U95 and P(-484), respectively. [Figure 10] Figure 10 depicts the effects of R2 deletion 20 on promoter activity. The upper left graph shows Jurkat cells, the upper right graph shows Molt-3 cells, the lower left graph shows SupT1 cells, and the lower right graph shows SAS-413 cells. The graphs show from the left,7MIE promoter (-493), 7MIE promoter (-388), 7MIE promoter (-233), 25 7U95 promoter (-484), 7U95 promoter (-379) and 7U95 promoter (-304). [Figure 11] Figure 11 depicts the promoter activity in a peripheral blood monocytic cell (PBMC). It shows lineage 1, linage 2 and lineage 3, in the upper left, upper right and 30 lower panels, respectively. BRIEF DESCRIPTION OF SEQUENCE LISTING -31 - OBK008 [0138] SEQ ID NO: 1 is the sequence of HHV6B MIE promoter. SEQ ID NO: 2 is the sequence of HHV7 MIE promoter. 5 SEQ ID NO: 3 is the sequence of HHV6A MIE promoter. SEQ ID NO: 4 is the sequence of HHV6B R3 region. SEQ ID NO: 5 is the sequence of 20u used in Example 1. SEQ ID NO: 6 is the sequence of 9u used in Example 1. SEQ ID NO: 7 is the sequence of MIE used in Example 1. 10 SEQ ID NO: 8 is the sequence of U95 used in Example 1. SEQ ID NO: 9 is the sequence of CMV used in Example 1. SEQ ID NO: 10 is the sequence of MIE/3K used in Example 1. SEQ ID NO: 11 is the sequence of U95/3K used in 15 Example 1. SEQ ID NO: 12 is the sequence of HHV7 U95 promoter SEQ ID NO: 13 is the sequence of -574 to -427 from the transcription initiation site of HHV6B MIE. SEQ ID NO: 14 is the sequence of -1051 to -427 from 20 the transcription initiation site of HHV6B MIE. SEQ ID NO: 15 is the sequence of +22 to -493 from the transcription initiation site of HHV7 MIE. SEQ ID NO: 16 is the sequence of +16 to -484 from the transcription initiation site of HHV7 MIE. 25 SEQ ID NO: 17 is the sequence of 9u-d2-7 used in Example 1. SEQ ID NO: 18 is the sequence of 9u-dl-4 used in Example 1. SEQ ID NO: 19 is the sequence of 9u-dl-5 used in 30 Example 1. SEQ ID NO: 20 is the sequence of 9u-dl-7 used in Example 1.

-32- OBKO08 SEQ ID NO: 21 is the sequence of 9u-d3-7 used in Example 1. SEQ ID NO: 22 is the sequence of 9u-d5 used in Example 1. 5 SEQ ID NO: 23 is the sequence of 9u-d6 used in Example 1. SEQ ID NO: 24 is the sequence of 9u-d7 used in Example 1. SEQ ID NO: 25 is the sequence of 9u-d8 used in 10 Example 1. SEQ ID NO: 26 is the sequence of 7MIEP (-493) used in Example 2. SEQ ID NO: 27 is the sequence of 7MIEP (-388) used in Example 2. 15 SEQ ID NO: 28 is the sequence of 7MIEP (-233) used in Example 2. SEQ ID NO: 29 is the sequence of 7U95P (-484) used in Example 2. SEQ ID NO: 30 is the sequence of 7U95P (-379) used in 20 Example 2. SEQ ID NO: 31 is the sequence of 7U95P (-304) used in Example 2. SEQ ID NO: 32 is the sequence of pGL3 Basic used in Example 2. 25 SEQ ID NO: 33 is an example of RNAi of HIV-1 gp4l. SEQ ID NO: 34 is an example of RNAi of HIV-1 tat.. SEQ ID NO: 35 is an example of RNAi of HIV-1 tax. BEST MODE FOR CARRYING OUT THE INVENTION 30 Hereinafter, the present invention will be described. It should be understood throughout the present -33- OBKO08 specification that articles for singular forms (e.g., "a", "an", "the", etc. in English, and articles, adjectives, etc. in other languages) include plural referents unless the context clearly dictates otherwise. It should be also 5 understood that the terms as used herein have definitions typically used in the art unless otherwise mentioned. Accordingly, unless otherwise defined, all terminology and technical terms used herein will have the same meanings as those generally understood by those skilled in the art 10 belonging to the filed of the present invention. If there is contradiction, the present specification (including the definition) takes precedence. [0140] (Definition of Terms) 15 The definitions of terms used herein are described below. [0141] As used herein the term "HHV" refers to a human herpes virus, of which there are types 1, 2, 3, 4, 5, 6, 7, 20 8 and the like. [0142] As used herein, the term "herpesvirus" includes all of HHV-6A, HHV-6B, and HHV-7, and both their wild-types and recombinant types unless otherwise mentioned. As used 25 herein, the term "HHV-6 (human herpes virus 6)" includes HHV-6A and HHV-6B, and both their wild-types and recombinant types unless otherwise mentioned. HHV6 belongs to the 8 subgenus as cytomegalovirus HHV-5, and HHV6B is a causative virus of exanthema subitum, and it is said that 30 most Japanese will have been infected therewith by the age of two years old. As used herein, the term "HHV-7 (human herpes virus 7)" refers to any herpes virus belonging to -34- OBKO08 this type of herpes virus. HHV7 is also said to be a causative body of exanthema subitum, however, in comparison to HHV6B, the occurrence thereof is lower, and the age where the patients are infected is older. As with HHV6, 5 HHV7 belongs to the 8 subgenus, and it is also said that it is believed to infect CD4 cells, and thus cause the onset of pityriasis rosea Gibert, and it is also said that most Japanese will have been infected therewith by the age of two years old. 10 [0143] As used herein, the term "wild strain" in relation to herpesvirus refers to a herpesvirus strain which is not artificially modified and is isolated from nature. An example of a wild strain includes, but is not 15 limited to, strain J1. [0144] As used herein, the term "wild strain" in relation to HHV-6A refers to a HHV-6A strain which is not artificially modified and is isolated from nature. An 20 example of a wild strain includes, but is not limited to, strain U1102. [0145] As used herein, the term "mutant strain" refers to a herpesvirus strain which has a mutation due to 25 mutagenesis, multiple subculturings or the like. Mutagenesis of a herpesvirus strain may be either random mutagenesis or site-specific mutagenesis. [0146] As used herein, the term "wild strain" in 30 relation to HHV-6B refers to a HHV-6B strain which is not artificially modified and is isolated from nature. An -35- OBKO08 example of a wild strain includes, but is not limited to, strain HST. [0147] The terms "protein", "polypeptide", 5 "oligopeptide" and "peptide" as used herein have the same meaning and refer to an amino acid polymer having any length. [0148] The terms "polynucleotide", "oligonucleotide", 10 and "nucleic acid" as used herein have the same meaning and refer to a nucleotide polymer having any length. Unless otherwise indicated, a particular nucleic acid sequence also implicitly encompasses conservatively-modified variants thereof (e.g. degenerate codon substitutions) and 15 complementary sequences as well as the sequence explicitly indicated. Specifically, degenerate codon substitutions may be produced by generating sequences in which the third position of one or more selected (or all) codons is substituted with mixed-base and/or deoxyinosine residues 20 (Batzer et al., Nucleic Acid Res. 19:5081(1991); Ohtsuka et al., J. Biol. Chem. 260:2605-2608 (1985); Rossolini et al., Mol. Cell. Probes 8:91-98(1994)). [0149] As used herein, the term "gene" refers to an 25 element defining a genetic trait. A gene is typically arranged in a given sequence on a chromosome. A gene which defines the primary structure of a protein is called a structural gene. A gene which regulates the expression of a structural gene is called a regulatory gene. As used 30 herein, "gene" may refer to "polynucleotide", "oligonucleotide", "nucleic acid", and "nucleic acid molecule" and/or "protein", "polypeptide", "oligopeptide" -36- OBKO08 and "peptide". As used herein, the term "open reading frame" or "ORF" in relation to a gene, refers to a reading frame which is one of three frames obtained by sectioning the base sequence of a gene at intervals of three bases, 5 and has a start codon and a certain length curtailed by the appearance of a stop codon, and has the possibility of actually coding a protein. The entire base sequence of the genome of herpesvirus has been determined, identifying at least 101 genes. Each of the genes is known to have an 10 open reading frame (ORF). [01501 As used herein, the term "RNAi" is an abbreviation of RNA interference and refers to a phenomenon where an agent for causing RNAi, such as double-stranded 15 RNA (also called dsRNA), is introduced into cells and mRNA homologous thereto is specifically degraded, so that the synthesis of gene products is suppressed, and techniques using the phenomenon. As used herein, RNAi may have the same meaning as that of an agent which causes RNAi. 20 [0151] As used herein, the term "an agent causing RNAi" refers to any agent capable of causing RNAi. As used herein, "an agent causing RNAi of a gene" indicates that the agent causes RNAi relating to the gene and that the 25 effect of RNAi is successfully achieved (e.g., suppression of expression of the gene, and the like). Examples of such an agent causing RNAi include, but are not limited to, a sequence having at least about 70% homology with the nucleic acid sequence of a target gene or a sequence 30 hybridizable thereto under stringent conditions, and RNA containing a double-stranded portion having a length of at least 10 nucleotides or variants thereof. Here, this agent -37- OBKO08 may be preferably DNA containing a 3' protruding end, and more preferably the 3' protruding end has a length of 2 or more nucleotides (e.g., 2-4 nucleotides in length). [0152] 5 Though not wishing to be bound by any theory, a mechanism which causes RNAi is considered to be as follows. When a molecule which causes RNAi, such as dsRNA, is* introduced into a cell, an RNaseIII-like nuclease having a helicase domain (called dicer) cleaves the molecule at 10 about 20 base pair intervals from the 3' terminus in the presence of ATP in the case where the RNA is relatively long (e.g., 40 or more base pairs). As used herein, the term "siRNA" is an abbreviation of short interfering RNA and refers to short double-stranded RNA of 10 or more base 15 pairs which are artificially chemically synthesized or biochemically synthesized, synthesized by an organism, or produced by double-stranded RNA of about 40 or more base pairs being degraded within the organism. siRNA typically has a structure comprising 5'-phosphate and 3'-OH, where 20 the 3' terminus projects by about 2 bases. A specific protein is bound to siRNA to form RISC (RNA-induced silencing-complex). This complex recognizes and binds to mRNA having the same sequence as that of siRNA and cleaves mRNA at the middle of siRNA due to RNaseIII-like enzymatic 25 activity. It is preferable that the relationship between the sequence of siRNA and the sequence of mRNA to be cleaved as a target is a 100% match. However, base mutations at a site away from the middle of siRNA do not completely remove the cleavage activity by RNAi, leaving 30 partial activity, while base mutations in the middle of siRNA have a large influence and the mRNA cleavage activity by RNAi is considerably lowered. By utilizing such a - 38 - OBKO08 characteristic, only mRNA having a mutation can be specifically degraded. Specifically, siRNA in which the mutation is provided in the middle thereof is synthesized and is introduced into a cell. Therefore, in the present 5 invention, siRNA per se, as well as an agent capable of producing siRNA (e.g., representatively dsRNA of about 40 or more base pairs) can be used as an agent capable of eliciting RNAi. [0153] 10 Also, though not wishing to be bound by any theory, apart from the above-described pathway, the antisense strand of siRNA binds to mRNA and siRNA functions as a primer for RNA-dependent RNA polymerase (RdRP), so that dsRNA is synthesized. This dsRNA is a substrate for a 15 dicer again, leading to production of new siRNA. It is intended that such a reaction is amplified. Therefore, in the present invention, siRNA per se, as well as an agent capable of producing siRNA are useful. In fact, in insects and the like, for example, 35 dsRNA molecules can 20 substantially or completely degrade 1,000 or more copies of intracellular mRNA, and therefore, it will be understood that siRNA per se, as well as an agent capable of producing siRNA, is useful. [0154] 25 In the present invention, double-stranded RNA having a length of about 20 bases (e.g. , representatively about 21 to 23 bases) or less than about 20 bases, called siRNA, can be used. Expression of siRNA in cells can suppress expression of a pathogenic gene targeted by the 30 siRNA. Therefore, siRNA can be used for the treatment, prophylaxis, prognosis, and the like of diseases. [0155] -39- OBKO08 The siRNA of the present invention may be in any form as long as it can elicit RNAi. [0156] In another embodiment, an agent capable of 5 causing RNAi may have a short hairpin structure having a sticky portion at the 3' terminus (shRNA; short hairpin RNA). As used herein, the term "shRNA" refers to a molecule of about 20 or more base pairs in which a single stranded RNA partially contains a palindromic base sequence 10 and forms a double-strand structure therein (i.e., a hairpin structure). shRNA can be artificially chemically synthesized. Alternatively, shRNA can be produced by linking sense and antisense strands of a DNA sequence in reverse directions and synthesizing RNA in vitro with T7 15 RNA polymerase using the DNA as a template. Though not wishing to be bound by any theory, it should be understood that after shRNA is introduced into a cell, the shRNA is degraded in the cell to a length of about 20 bases (e.g., representatively 21, 22, 23 bases), and causes RNAi as with 20 siRNA, leading to the treatment effects of the present invention. It should be understood that such an effect is exhibited in a wide range of organisms, such as insects, plants, animals (including mammals), and the like. Thus, shRNA elicits RNAi as with siRNA and therefore can be used 25 as an effective component of the present invention. shRNA may preferably have a 3' protruding end. The length of the double-stranded portion is not particularly limited, but is preferably about 10 or more nucleotides, and more preferably about 20 or more nucleotides. Here, the 3' 30 protruding end may be preferably DNA, more preferably DNA of at least 2 nucleotides in length, and even more preferably DNA of 2-4 nucleotides in length.

-40- OBKO08 [0157] An agent capable of causing RNAi used in the present invention may be artificially synthesized (chemically or biochemically) or naturally occurring. 5 There is substantially no difference between the two in terms of the effect of the present invention. A chemically synthesized agent is preferably purified by liquid chromatography or the like. [01581 10 An agent capable of causing RNAi used in the present invention can be produced in vitro. In this synthesis system, T7 RNA polymerase and T7 promoter are used to synthesize antisense and sense RNAs from template DNA. These RNAs are annealed and thereafter introduced 15 into a cell. In this case, RNAi is caused via the above described mechanism, thereby achieving the effect of the present invention. Here, for example, the introduction of RNA into a cell can be carried out using a calcium phosphate method. 20 [0159] Another example of an agent capable of causing RNAi according to the present invention is a single stranded nucleic acid hybridizable to mRNA, or all nucleic acid analogs thereof. Such agents are useful for the 25 method and composition of the present invention. [0160] As used herein, the term "corresponding" amino acid or nucleic acid refers to an amino acid or nucleotide in a given polypeptide or polynucleotide molecule, which 30 has, or is anticipated to have, a function similar to that of a predetermined amino acid or nucleotide in a polypeptide or polynucleotide as a reference for comparison.

-41 - OBKO08 For example, in the case of ubiquitin, it refers to an amino acid contributing in a similar manner to the catalytic activity and present in a similar location as in the sequence (for example, glycine at the C-terminus) which 5 is responsible for lysine. For example, in the case of nucleic acid sequence, the term refers to a similar portion which affects a similar function to the particular portion which it encodes. [0161] 10 As used herein, the term "corresponding" gene (e.g., a polypeptide or polynucleotide molecule) refers to a gene in a given species, which has, or is anticipated to have, a function similar to that of a predetermined gene in a species as a reference for comparison. When there are 15 pluralities of genes having such a function, the term refers to a gene having the same evolutionary origin. Therefore, a gene corresponding to a given gene may be an ortholog of the given gene. Therefore, genes corresponding to those such as herpes virus type 6B and tumor antigen and 20 the like, can be found in other organisms (for example, herpes virus type 7). Such a corresponding gene can be identified by techniques well known in the art. Therefore, for example, a corresponding gene in a given organism can be found by searching a sequence database of the organism 25 (e.g., herpes virus 6B) using the sequence of a reference gene (e.g., mouse cyclin gene, etc.) as a query sequence. Alternatively, wet experiments are used for screening a library to find out the same. [0162] 30 As used herein, the term "isolated" means that naturally accompanying material is at least reduced, or preferably substantially or completely eliminated, in -42- OBKO08 normal circumstances. Therefore, the term "isolated cell" refers to a cell substantially free from other accompanying substances (e.g., other cells, proteins, nucleic acids, etc. ) in natural circumstances. The term "isolated" in 5 relation to nucleic acids or polypeptides means that, for example, the nucleic acids or the polypeptides are substantially free from cellular substances or culture media when they are produced by recombinant DNA techniques; or precursory chemical substances or other chemical 10 substances when they are chemically synthesized. [0163] As used herein, the term "purified" biological agent (e.g., nucleic acids, proteins, and the like) refers to one from which at least a portion of naturally 15 accompanying agents has been removed. Therefore, ordinarily, the purity of a purified biological agent is higher than that of the biological agent in a normal state (i.e., concentrated). [0164] 20 As used herein, the terms "purified" and "isolated" mean that the same type of biological agent is present preferably at least 75% by weight, more preferably at least 85% by weight, even more preferably at least 95% by weight, and most preferably at least 98% by weight. 25 [0165] As used herein, the term "homology" in relation to a sequence (e.g., a nucleic acid sequence, an amino acid sequence, etc.) refers to the proportion of identity between two or more gene sequences. Therefore, the greater 30 the homology between two given genes, the greater the identity or similarity between their sequences. Whether or not two genes have homology is determined by comparing -43- OBK008 their sequences directly or by a hybridization method under stringent conditions. When two gene sequences are directly compared with each other, these genes have homology if the DNA sequences of the genes have representatively at least 5 50% identity, preferably at least 70% identity, more preferably at least 80%, 90%, 95%, 96%, 97%, 98%, or 99% identity with each other. [0166] As used herein, "polynucleotides hybridizing 10 under stringent conditions" refers to conditions commonly used and well known in the art. Such a polynucleotide can be obtained by conducting colony hybridization, plaque hybridization, Southern blot hybridization, or the like using a polynucleotide selected from the polynucleotides of 15 the present invention. Specifically, a filter on which DNA derived from a colony or plaque is immobilized is used to conduct hybridization at 65 0 C in the presence of 0.7 to 1.0 M NaCl. Thereafter, a 0.1 to 2-fold concentration SSC (saline-sodium citrate) solution (1-fold concentration SSC 20 solution is composed of 150 mM sodium chloride and 15 mM sodium citrate) is used to wash the filter at 65 0 C. Polynucleotides identified by this method are referred to as "polynucleotides hybridizing under stringent conditions". Hybridization can be conducted in accordance with a method 25 described in, for example, Molecular Cloning 2nd ed., Current Protocols in Molecular Biology, Supplement 1-38, DNA Cloning 1: Core Techniques, A Practical Approach, Second Edition, Oxford University Press (1995), and the like. Here, sequences hybridizing under stringent 30 conditions exclude, preferably, sequences containing only A or T. "Hybridizable polynucleotide" refers to a polynucleotide which can hybridize to other polynucleotides -44- OBKO08 under the above-described hybridization conditions. Specifically, the hybridizable polynucleotide includes at least a polynucleotide having a homology of at least 60% to the base sequence of DNA encoding a polypeptide having an 5 amino acid sequence specifically herein disclosed, preferably a polynucleotide having a homology of at least 80%, and more preferably a polynucleotide having a homology of at least 95%. [0167] 10 The similarity, identity and homology of amino acid sequences and base sequences are herein compared using FASTA with the default parameters. Alternatively, an identity search may be conducted, for example, using NCBI's BLAST 2.2.9 (published May 12, 2004). As used herein, the 15 value of identity usually refers to the value as a result of alignment with the BLAST as described above using the default parameters. If the change of parameters results in higher values, then the highest value is employed herein as the value of the identity. When a plurality of regions are 20 evaluated for identity, the highest value is employed herein as the value of the identity. [0168] As used herein, the term "search" indicates that a given nucleic acid sequence is utilized to find 25 other nucleic acid base sequences having a specific function and/or property either electronically or biologically, or using other methods. Examples of an electronic search include, but are not limited to, BLAST (Altschul et al., J. Mol. Biol. 215:403-410 (1990)), FASTA 30 (Pearson & Lipman, Proc. Natl. Acad. Sci., USA 85:2444-2448 (1988)), Smith and Waterman method (Smith and Waterman, J. Mol. Biol. 147:195-197 (1981)), and Needleman and Wunsch -45- OBKO08 method (Needleman and Wunsch, J. Mol. Biol. 48:443-453 (1970)), and the like. Examples of a biological search include, but are not limited to, a macroarray in which genomic DNA is attached to a nylon membrane or the like or 5 a microarray (microassay) in which genomic DNA is attached to a glass plate under stringent hybridization, PCR and in situ hybridization, and the like. As used herein, it is intended that promoters used in the present invention encompass a sequence corresponding to those identified by 10 such an electronic or biological search. [0169] As used herein, the term "expression" of a gene product, such as a gene, a polynucleotide, a polypeptide, or the like, indicates that the gene or the like is 15 affected by a predetermined action in vivo to be changed into another form. Preferably, the term "expression" indicates that genes, polynucleotides, or the like are transcribed and translated into polypeptides. In one embodiment of the present invention, genes may be 20 transcribed into mRNA. More preferably, these polypeptides may have post-translational processing modifications. [0170] As used herein amino acids may be referred to with the generally known three-letter abbreviation or the 25 one letter-abbreviation proposed by the IUPAC-IUB Biochemical Nomenclature Commission. Nucleotides may also be referred to with the generally known one-letter abbreviations which are generally accepted. [0171] 30 The letter codes are as follows: Amino Acids: 3-letter single-letter reference -46- OBKOO8 Ala A alanine Cys C cysteine Asp D aspartic acid Glu E glutamic acid 5 Phe F phenylalanine Gly G glycine His H histidine Ile I isoleucine Lys K lysine 10 Leu L leucine Met M methionine Asn N asparagine Pro P proline Gln Q glutamine 15 Arg R arginine Ser S serine Thr T threonine Val V valine Trp W tryptophane 20 Tyr Y tyrosine Asx asparatic acid or asparagine Glx glutamine or glutamic acid Xaa unknown or other amino acid [0172] 25 Base (Nucleotide) abbreviation reference a adenine g guanine 30 c cytosine t thymine u uracyl -47- OBKO08 r guanine or adenine purine y thymine/uracil or cytosine purimidine m adenin or cytocine amino group k guanine or thymine uracil keto group 5 s guanin or cytosine w adenine or thymine/uracil b guanine or cytocine or thymine/uracil d adenine or guanine or thymine/uracil h adenine or cytosine or thymine/uracil 10 V adenine or guanine or cytosine n adenine or guanine or cytosine or thymine/uracil, unknown or other base [0173] As used herein, the term "fragment" with 15 respect to a polypeptide or polynucleotide refers to a polypeptide or polynucleotide having a sequence length ranging from 1 to n-1 with respect to the full length of the reference polypeptide or polynucleotide (of length n). The length of the fragment can be appropriately changed 20 depending on the purpose. For example, in the case of polypeptides, the lower limit of the length of the fragment includes 3, 4, 5, 6, 7, 8, 9, 10, 15, 20, 25, 30, 40, 50 or more nucleotides. Lengths represented by integers which are not herein specified (e.g., 11 and the like) may be 25 appropriate as a lower limit. For example, in the case of polynucleotides, the lower limit of the length of the fragment includes 5, 6, 7, 8, 9, 10, 15, 20, 25, 30, 40, 50, 75, 100, 200, 300, 400, 500, 600, 700, 800, 900, 1000 or more nucleotides. Lengths represented by integers which 30 are not herein specified (e.g., 11 and the like) may be appropriate as a lower limit. [0174] -48 - OBKO08 A polypeptide used in the present invention may have at least one (for example, one or several or more) amino acid substitutions, addition and/or deletion in the amino acid sequence, as long as it has substantially identical 5 function as the wild type polypeptide. [0175] It is well known that if a given amino acid is substituted with another amino acid having a similar hydrophobicity index, the resultant protein may still have 10 a biological function similar to that of the original protein (e.g., a protein having an equivalent enzymatic activity). For such an amino acid substitution, the hydrophobicity index is preferably within 2, more preferably within ±1, and even more preferably within ±0.5. 15 It is understood in the art that hydrophobicity is considered in the modification of a protein. As described in US Patent No. 4,554,101, amino acid residues are given the following hydrophilicity indices: arginine (+3.0); lysine (+3.0); aspartic acid (+3.0±1); glutamic acid 20 (+3.0±1); serine (+0.3); asparagine (+0.2); glutamine (+0.2); glycine (0); threonine (-0.4); proline (-0.5±1); alanine (-0.5); histidine (-0.5); cysteine (-1.0); methionine (-1.3); valine (-1.5); leucine (-1.8); isoleucine (-1.8); tyrosine (-2.3); phenylalanine (-2.5); 25 and tryptophan (-3.4). It is understood that an amino acid may be substituted with another amino acid which has a similar hydrophilicity index and can still provide a biological equivalent. For such an amino acid substitution, the hydrophilicity index is preferably within 2, more 30 preferably ± 1, and even more preferably ±0.5. A hydrophilicity index is also useful for modification of an amino acid sequence of the present invention. As described -49- OBK008 in US Patent No. 4,554,101, amino acid residues are given the following hydrophilicity indices: arginine (+3.0); lysine (+3.0); aspartic acid (+3.0±1); glutamic acid (+3.0±1); serine (+0.3); asparagine (+0.2); glutamine 5 (+0.2); glycine (0); threonine (-0.4); proline (-0.5±1); alanine (-0.5); histidine (-0.5); cysteine (-1.0); methionine (-1.3); valine (-1.5); leucine (-1.8); isoleucine (-1.8); tyrosine (-2.3); phenylalanine (-2.5); and tryptophan (-3.4). It is understood that an amino acid 10 may be substituted with another amino acid which has a similar hydrophilicity index and can still provide a biological equivalent. For such an amino acid substitution, the hydrophilicity index is preferably within ±2, more preferably ± 1, and even more preferably ±0.5. 15 [0176] The term "conservative substitution" as used herein refers to an amino acid substitution in which a substituted amino acid and a substituting amino acid have similar hydrophilicity indices or/and hydrophobicity 20 indices. For example, the conservative substitution is carried out between amino acids having a hydrophilicity or hydrophobicity index of within ±2, preferably within 1, and more preferably within ±0.5. Examples of conservative substitution include, but are not limited to, substitutions 25 within each of the following residue pairs: arginine and lysine; glutamic acid and aspartic acid; serine and threonine; glutamine and asparagine; and valine, leucine, and isoleucine, which are well known to those skilled in the art. 30 [0177] As used herein, the term "variant" refers to a substance, such as a polypeptide, polynucleotide, or the -50- OBK008 like, which differs partially from the original substance. Examples of such a variant include a substitution variant, an addition variant, a deletion variant, a truncated variant, an allelic variant, and the like. Examples of 5 such a variant include, but are not limited to, a nucleotide or polypeptide having one or several substitutions, additions and/or deletions or a nucleotide or polypeptide having at least one substitution, addition and/or deletion. The term "allele" as used herein refers 10 to a genetic variant located at a locus identical to a corresponding gene, where the two genes are distinguishable from each other. Therefore, the term "allelic variant" as used herein refers to a variant which has an allelic relationship with a given gene. Such an allelic variant 15 ordinarily has a sequence the same as or highly similar to that of the corresponding allele, and ordinarily has almost the same biological activity, though it rarely has different biological activity. The term "species homolog" or "homolog" as used herein refers to one that has an amino 20 acid or nucleotide homology with a given gene in a given species (preferably at least 60% homology, more preferably at least 80%, at least 85%, at least 90%, and at least 95% homology). A method for obtaining such a species homolog is clearly understood from the description of the present 25 specification. The term "orthologs" (also called orthologous genes) refers to genes in different species derived from a common ancestry (due to speciation). For example, in the case of the hemoglobin gene family having multigene structure, human and mouse a-hemoglobin genes 30 are orthologs, while the human a-hemoglobin gene and the human p-hemoglobin gene are paralogs (genes arising from gene duplication). Orthologs are useful for estimation of -51- OBKO08 molecular phylogenetic trees. Usually, orthologs in different species may have a function similar to that of the original species. Therefore, orthologs of the present invention may be useful in the present invention. 5 [0178] As used herein the term "functional variant" refers to a variant which retains a biological activity (in particular, promoter activity" which the sequence of standard is responsible for. 10 [0179] As used herein, the term "conservative (or conservatively modified) variant" applies to both amino acid and nucleic acid sequences. With respect to particular nucleic acid sequences, conservatively modified variants 15 refer to those nucleic acids which encode identical or essentially identical amino acid sequences. Because of the degeneracy of the genetic code, a large number of functionally identical nucleic acids encode any given protein. For example, the codons GCA, GCC, GCG and GCU all 20 encode the amino acid alanine. Thus, at every position where an alanine is specified by a codon, the codon can be altered to any of the corresponding codons described without altering the encoded polypeptide. Such nucleic acid variations are "silent variations" which represent one 25 species of conservatively modified variation. In a nucleic acid, a conservative substitution can be confirmed by measuring promoter activity, for example. [01801 In order to prepare functionally equivalent 30 polypeptides, amino acid additions, deletions, or modifications can be performed in addition to amino acid substitutions. Amino acid substitution(s) refers to the -52- OBKO08 replacement of at least one amino acid of an original peptide with different amino acids, such as the replacement of 1 to 10 amino acids, preferably 1 to 5 amino acids, and more preferably 1 to 3 amino acids with different amino 5 acids. Amino acid addition(s) refers to the addition of at least one amino acid to an original peptide chain, such as the addition of 1 to 10 amino acids, preferably 1 to 5 amino acids, and more preferably 1 to 3 amino acids to an original peptide chain. Amino acid deletion(s) refers to 10 the deletion of at least one amino acid, such as the deletion of 1 to 10 amino acids, preferably 1 to 5 amino acids, and more preferably 1 to 3 amino acids. Amino acid modification includes, but is not limited to, amidation, carboxylation, sulfation, halogenation, truncation, 15 lipidation, alkylation, glycosylation, phosphorylation, hydroxylation, acylation (e.g., acetylation), and the like. Amino acids to be substituted or added may be naturally occurring or nonnaturally-occurring amino acids, or amino acid analogs. Naturally-occurring amino acids are 20 preferable. [0181] Nucleic acid embodiment of the polypeptide to be expressed as used herein refers to a nucleic acid which allows expression of the protein embodiment of the polypeptide. Such a nucleic acid 25 includes one in which a part of the sequence of the nucleic acid is deleted or is substituted with other base(s), or an additional nucleic acid sequence is inserted, as long as a polypeptide expressed by the nucleic acid has substantially the same activity as that of the naturally-occurring 30 polypeptide, as described above. Alternatively, an additional nucleic acid may be linked to the 5' terminus and/or 3' terminus of the nucleic acid. The nucleic acid -53- OBKO08 molecule may include one that is hybridizable to a gene encoding a polypeptide under stringent conditions and encodes a polypeptide having substantially the same function as that of that polypeptide. Such a gene is known 5 in the art and can be used in the present invention. [0182] The above-described nucleic acid can be obtained by a well-known PCR method, i.e., chemical synthesis. This method may be combined with, for example, 10 site-specific mutagenesis, hybridization, or the like. [0183] As used herein, the term "substitution, addition or deletion" for a polypeptide or a polynucleotide refers to the substitution, addition or deletion of an 15 amino acid or its substitute, or a nucleotide or its substitute with respect to the original polypeptide or polynucleotide. This is achieved by techniques well known in the art, including a site-specific mutagenesis technique and the like. A polypeptide or a polynucleotide may have 20 any number (>0) of substitutions, additions, or deletions. The number can be as large as a variant having such a number of substitutions, additions or deletions can maintain an intended function (e.g., the information transfer function of hormones and cytokines, etc.). For 25 example, such a number may be one or several, and preferably within 20% or 10% of the full length sequence, or no more than 100, no more than 50, no more than 25, or the like. [0184] 30 (promoter) As used herein, the term "promoter (or promoter sequence)" refers to a base sequence which determines the -54- OBKO08 initiation site of transcription of a gene and is a DNA region which directly regulates the frequency of transcription. Transcription is started by RNA polymerase binding to a promoter. Accordingly, as used herein a 5 portion having the function of a promoter of a gene refers to "a promoter portion". A promoter region can be deduced by predicting the protein coding region in a genomic base sequence using DNA analysis software. Deduced promoter regions are usually located upstream of the structural gene 10 although it varies, and is not limited thereto, and may also be downstream of the structural gene. (01851 As used herein, the term "MIE promoter" refers to a major immediate early promoter, which is a promoter of a 15 gene which is immediately transcribed by a transcription factor derived from a host and a virion after viral infection. The MIE gene may be identified by RT-PCR using an RNA extracted from an infected cell treated with cycloheximide. 20 [0186] As used herein, the term "U95 promoter" refers to a promoter of the immediate early gene U95. U95 is also an immediate early gene, and thus is immediately transcribed by a transcription factor derived from a host or a virion 25 after the viral infection. [0187] As used herein, the identification method of a promoter is as follows: some sequences in the vicinity of the structural gene are screened (for example, using an 30 expression cassette described in the Examples), and the sequence having the gene expression promoting activity is mapped. As such, a sequence having significant promoting -55- OBKO08 activity may be identified. Usually, it is located upstream of the structural gene, but is not limited thereto. [0188] As used herein, the term "HHV6B MIE promoter" or "MIE 5 promoter of HHV6B" refers to any sequence having promoter activity in SEQ ID NO: 1. Preferably, the promoter has position -814 to position 0 from the transcription initiation point in SEQ ID NO: 1. Such a sequence includes, but is not limited to SEQ ID NO: 1 or a sequence 10 corresponding thereto. In the expression control of HHV6B gene, it is preferable to be located in the region at -574 to -427 from the upstream, and preferably, in the region of -1051 to -427, and the base sequence thereof includes sequences set forth in SEQ ID NO: 15, 16 and the like. 15 Amongst them, it has been elucidated herein that NF-K B and AP-1 motifs (-603 to -594 from the transcription initiation point as the origin, corresponds to NF-K B motif, and -488 to -478 and -249 to -239 correspond to the AP-1 motifs.) may be motifs from experiments of base sequence 20 substitution. Accordingly, preferably, the HHV6B MIE promoter of the present invention comprises: (a) a polynucleotide having the base sequence set forth in SEQ ID NO: 1, or the base sequence corresponding thereto or a fragment sequence thereof; (b) a polynucleotide of an 25 allelic variant of the base sequence set forth in SEQ ID NO: 1 or the base sequence corresponding thereto or a fragment sequence thereof; (c) a polynucleotide which hybridizes a polynucleotide of any of (a) or (b) and has a biological activity thereof; or (d) a polynucleotide which 30 consists of the base sequence of any of (a) to (c) or a complement sequence thereof with at least 70 % identity, and has a biological activity thereof.

-56- OBK008 [0189] As used herein, the term "HHV7 MIE promoter" or "MIE promoter of HHV7" refers to any sequence having promoter activity in SEQ ID NO: 2. Preferably, the promoter has 5 position -493 to position +22 from the transcription initiation point in SEQ ID NO: 2. Such a sequence includes, but is not limited to SEQ ID NO: 2 or a sequence corresponding thereto. In the expression control of the HHV7 gene, it is preferable to be located in the region at 10 427 from the upstream, and preferably, in the region of 493, and the base sequence thereof includes sequences set forth in SEQ ID NO: 2 and the like. Amongst them, it has been elucidated herein that NF-KB motifs (-464 to -478 and -359 to -350 from the transcription initiation point as the 15 origin, corresponds to NF-KB motifs) may be motifs from experiments of base sequence substitution. Accordingly, preferably, the HHV7 MIE promoter of the present invention comprises: (a) a polynucleotide having the base sequence set forth in SEQ ID NO. 2, or the base sequence 20 corresponding thereto or a fragment sequence thereof; (b) a polynucleotide of an allelic variant of the base sequence set forth in SEQ ID NO. 2 or the base sequence corresponding thereto or a fragment sequence thereof; (c) a polynucleotide which hybridizes a polynucleotide of any of 25 (a) or (b) and has a biological activity thereof; or (d) a polynucleotide which consists of the base sequence of any of (a) to (c) or a complement sequence thereof with at least 70 % identity, and has a biological activity thereof. [0190] 30 As used herein, the term "HHV7 U95 promoter" or "U95 promoter of HHV7" refers to any sequence having promoter activity in SEQ ID NO: 12. Preferably, the promoter has -57 - OBKO08 position -484 to position +16 from the transcription initiation point in SEQ ID NO: 12. In the expression control of the HHV7 gene, it is preferable to be located in the region at -379 from the upstream, and preferably, in 5 the region of -484, and the base sequence thereof includes sequences set forth in SEQ ID NO: 2 and the like. Amongst them, it has been elucidated herein that NF-KB motifs (-478 to -469 and -373 to -364 from the transcription initiation point as the origin, correspond to NF-KB motifs) may be 10 motifs from experiments of base sequence substitution. Accordingly, preferably, the HHV7 U95 promoter of the present invention comprises: (a) a polynucleotide having the base sequence set forth in SEQ ID NO. 12, or the base sequence corresponding thereto or a fragment sequence 15 thereof; (b) a polynucleotide of an allelic variant of the base sequence set forth in SEQ ID NO. 12 or the base sequence corresponding thereto or a fragment sequence thereof; (c) a polynucleotide which hybridizes a polynucleotide of any of (a) or (b) and has a biological 20 activity thereof; or (d) a polynucleotide which consists of the base sequence of any of (a) to (c) or a complement sequence thereof with at least 70 % identity, and has a biological activity thereof. [0191] 25 "Constitutive" expression of a gene by a promoter of the present invention as used herein refers to a trait in which expression is found at a substantial but unchanged amount in any tissue of an organism during any stage in the course of the growth of the organism. 30 Specifically, when northern blot analysis is carried out under conditions similar to those in the examples described herein, if substantial and similar expression is observed -58- OBKO08 in the same or corresponding site thereof on any time points (e.g. two or more time points such as day 5 and day 15), the expression is regarded as being constitutive by the definition in the present invention. Constitutive 5 promoters are believed to play a role in the homeostasis of organisms in a normal growth environment. These traits can be determined by extracting RNA from an arbitrary portion and subjecting the RNA to northern blot analysis to analyze expression amounts. 10 [0192] "Enhancer" may be used so as to enhance the expression efficiency of a gene of interest. As such an enhancer, an enhancer region containing an upstream sequence within the CaMV35S promoter is preferable. A 15 plurality of enhancers or a single enhancer may be used, or no enhancer may be used. A region in a promoter which enhances the activity of the promoter may also be referred to as an enhancer. [0193] 20 As used herein, "operatively linked" or "operative link" refers to the fact that the expression (operation) of a desired sequence is located under the control of a transcription regulation sequence (e.g. promoter, enhancer or the like) or a translation regulation sequence. In 25 order that a promoter is operably linked to a gene, the promoter is usually located immediately upstream of the gene, but is not necessarily located in a flanking manner. [0194] (Nucleic acid construct) 30 As used herein, the term "nucleic acid construct" or "gene cassette" are interchangeably used to refer to a nucleic acid sequence comprising nucleic acid (for example, - 59 - OBKO08 DNA, RNA) encoding a gene, a nucleic acid sequence comprising a gene promoter operably linked thereto (such that it can control the expression of the nucleic acid), a promoter, and optionally a heterologous gene operably 5 linked thereto (i.e., in frame). It is intended that the use of this cassette or the construct optionally in combination with another regulatory element is encompassed in the present invention. Preferably expression cassettes or nucleic acid constructs are those which are amenable to 10 specific restriction enzyme digestion and are feasible for recovery. [0195] When a gene is mentioned herein, the term "recombinant vector" refers to a vector transferring a 15 polynucleotide sequence of interest to a target cell. Such a vector is capable of self-replication or incorporation into a chromosome of a host cell (e.g., a prokaryotic cell, yeast, an animal cell, a plant cell, an insect cell, an individual animal, and an individual plant, etc.), and 20 contains a promoter at a site suitable for transcription of a polynucleotide of the present invention. In the present application, for example, BAC vectors may be used. BAC vector refers to a plasmid produced based on the F plasmid of an E.coli, and is capable of propagating and stably 25 maintaining a DNA fragment of about 300kb or greater in size, in a bacteria such as E.coli or the like. BAC vector comprises at least a region essential for replication of BAC vectors. Such a region essential for replication includes, for example, oriS, a replication initiation point 30 of F plasmid, or a variant thereof. [01961 -60- OBKO08 As used herein, "selective marker" refers to a gene which functions as guidance for selecting a host cell comprising a nucleic acid construct or a vector. Selective markers include, but are not limited to: fluorescent 5 markers, luminescent markers and drug selective markers. "Fluorescent markers" include, but are not limited to gene encoding fluorescence proteins such as green fluorescent protein (GFP), cyan fluorescent protein (CFP), yellow fluorescent protein (YFP), red fluorescent protein (dsRFP). 10 "Luminescent markers" include but are not limited to genes encoding luminescent proteins such as luciferases. "Drug selective markers" include but are not limited to: hypoxanthine guanine phosphoribosyl transferase (hprt), dihydrofolate reductase gene, glutamine synthase gene, 15 aspartate transaminase, metallothionein (MT), adenosine aminase (ADA), AMP deaminase (AMPD1,2), xanthine-guanine phosphoribosyl transferase, UMP synthase, P-glycoprotein, asparagine synthase, and ornithine decarboxylase. A combination of a drug in conjunction with these drug 20 selective markers including those encoding proteins, for example: the combination of dihydrofolate reductase (DHFR) gene and methotrexate (MTX); the combination of glutamine synthase (GS) gene and methionine sulfoximine (Msx); the combination of aspartate transaminase (AST) gene and N 25 phosphone acetyl-L-aspartate (PALA); the combination of MT gene and cadmium (Cd 2 ); the combination of adenosine deaminase (ADA) gene and adenosine, alanosine, 2' deoxycoformycin; the combination of AMP deaminase (AMPD1.2) gene and adenine, azaserine and coformycin; the combination 30 of xanthine-guanine-phosphoribosyl transferase gene and mycophenolic acid; the combination of UMP synthase gene and 6-azauridine, pyrazofuran; the combination of P- -61- OBKO08 glycoprotein (P-gp, MDR) gene and multi drugs; the combination of aspartate synthase (AS) gene and B-aspartyl hydroxamic acid or albizziin; ornithine carboxylase (ODC) gene and a-difluoromethyl-ornithine 5 (DFMO) and the like. [0197] As used herein, the term "expression vector" refers to a nucleic acid sequence comprising a structural gene and a promoter for regulating expression thereof, and 10 in addition, various regulatory elements in a state that allows them to operate within host cells. The regulatory element may include, preferably, terminators, selectable markers such as drug-resistance genes (e.g. kanamycin resistant gene, hygromycin resistant gene and the like), 15 and enhancers. It is well known in the art that a type of expression vector of a living organism such as an animal and a species of a regulatory element used may vary depending on the type of host cell used. [01981 20 As used herein, the term "recombinant vector" refers to a vector transferring a polynucleotide sequence of interest to a target cell. Such a vector is capable of self-replication or incorporation into a chromosome in a host cell (e.g., a prokaryotic cell, yeast, an animal cell, 25 a plant cell, an insect cell, an individual animal, and an individual plant, etc.), and contains a promoter at a site suitable for transcription of a polynucleotide of the present invention. [0199] 30 As used herein, the term "terminator" refers to a sequence which is located downstream of a protein encoding region of a gene and which is involved in the - 62- OBKO08 termination of transcription when DNA is transcribed into mRNA, and the addition of a poly-A sequence. It is known that a terminator contributes to the stability of mRNA, and has an influence on the amount of gene expression. 5 Terminators include, but are not limited to, a sequence including AATAAA. [0200] As used herein, the term "foreign gene" to a particular organism refers to a gene which does not 10 natively exist in the particular organism. Such a foreign gene may be a gene modified from a gene which naturally occurs in the particular organism, or a gene which naturally occurs in an organism that is different from the particular organism (such as ADA gene), or an artificially 15 synthesized gene, or a complex thereof such as a fusion. An organism comprising such a foreign gene may express a genetic product which is not expressed in nature. For example, a recessive gene to be deleted (for example, ADA gene, PNP gene, y c chain gene, TAP gene, MHC II gene, X 20 linked WASP, CD40 ligand, P13K-like gene, DNA helicase) may be used as a foreign gene. [0201] As used herein, the foreign gene may be a gene of a cytokine. As used herein, the term "cytokine" is defined 25 as in the broadest sense used in the art, and a physiologically active substance which is produced from a cell and acts on the same cell or a different cell. Cytokines are generally a protein or a polypeptide, and have a controlling action of immunological response, 30 regulation of endocrine system, regulation of the nerve system, antitumor activity, antiviral activity, regulation of cell proliferation, regulation of cellular -63- OBKO08 differentiation and the like. As used herein, cytokines may exist in a form of protein or nucleic acid, and at the actual time of action, cytokines usually mean a protein form. As used herein, the term "growth factor" refers to a 5 substance which promotes or controls the growth of a cell. Growth factors may substitute the action of serum macromolecular substances by addition to a medium in cell culture or tissue culture. Many growth factors have been found to function as a regulation factor of a 10 differentiation state other than growth of a cell. Cytokines typically include interleukins, chemokines, hematopoietic factors such as colony stimulation factors, tumor necrosis factors, interferons. Growth factors typically include platelet derived growth factor (PDGF), 15 epidermal growth factor (EGF), fibroblast growth factor (FGF), hepatocytic growth factor (HGF), vessel endothelial growth factor (VEGF), and the like, which show growth activity. [0202] 20 In the present invention, those having homology with a foreign gene of a native form as described above may be used as a foreign gene to be expressed. Such foreign genes having such homology include, but are not limited to: for example, when conducting comparison using default 25 parameters of Blast in comparison to a foreign gene of reference to be compared, nucleic acids having sequences of identity or similarity of at least about 30 %, at least about 35 %, at least about 40 %, at least about 30 %, at least about 45 %, at least about 50 %, at least about 55 %, 30 at least about 60 %, at least about 65 %, at least about 70 %, at least about 75 %, at least about 80 %, at least about 85 %, at least about 90 %, at least about 95 %, at -64- OBKO08 least about 99 %, or polypeptides having amino acid sequence of identity or similarity of at least about 30 %, at least about 35 %, at least about 40 %, at least about 30 %, at least about 45 %, at least about 50 %, at least 5 about 55 %, at least about 60 %, at least about 65 %, at least about 70 %, at least about 75 %, at least about 80 %, at least about 85 %, at least about 90 %, at least about 95 %, at least about 99 %. [0203] 10 As used herein, the term "expression" of a gene product, such as a gene, a polynucleotide, a polypeptide, or the like, indicates that the gene or the like is affected by a predetermined action in vivo to be changed into another form. Preferably, the term "expression" 15 indicates that genes, polynucleotides, or the like are transcribed and translated into polypeptides. In one embodiment of the present invention, genes may be transcribed into mRNA. More preferably, these polypeptides may have post-translational processing modifications. 20 [0204] Accordingly, as used herein, "reduction" of "expression" of a gene, a polynucleotide, a polypeptide or the like refers to when an agent of the present invention is subjected to an action, whereby the amount of expression 25 is significantly reduced compared to that when the agent is not subjected to an action. Preferably, the reduction of expression includes a reduction of the level of polypeptide expression. As used herein, the "increase" of "expression" of a gene, a polynucleotide, a polypeptide or the like 30 refers to when an agent of the present invention is subjected to an action (or an agent relating to gene expression into a cell, for example, a gene to be expressed -65- OBKO08 or an agent for regulating the same), whereby the amount of expression is significantly increased compared to when the agent is not subjected to an action. Preferably, the increase of expression includes an increase in the level of 5 polypeptide expression. As used herein, the term "induction" of "expression" of a gene refers to an increase in the level of expression of the gene by acting an agent on a cell. Accordingly, the induction of expression encompasses when the level of expression of the gene is 10 observed to increase from an observed level of no expression, to a noticeable level of expression of the gene. [0205] As used herein, the term "specifically express(ing)" of a gene refers to expression in a different 15 level (preferably in a higher level) in a specific site or period of time than that of the other site or period of time. Specific expression may refer to expression in a certain site (specific site) or may also refer to the expression including that in another site. Preferably, 20 specific expression refers to the expression in the certain site only. [0206] Methods of introducing a recombinant vector are also achieved by any of the above-mentioned methods for 25 introducing DNA into a cell, and include for example, transfection, transduction, transformation and the like, such as calcium phosphate, liposome methods, DEAE dextran methods, electroporation methods, particle gun methods (gene gun), and the like, lipofection, spheroplast Proc. 30 Natl. Acad. Sci. USA, 84, 1929 (1978)], lithium acetate method [J. Bacteriol., 153, 163 (1983)], a method described in Proc. Natl. Acad. Sci. USA, 75, 1929 (1978) and the like.

-66- OBKO08 [0207] Transitional expression of Cre enzyme, DNA mapping on the chromosomes and the like, used in a method for removing a genome or genomic locus used herein or the like are well 5 known in the art as described in "FISH jikken purotokooru hito/genomu kaiseki kara senshokutai/idenshi shindan made (FISH Experimental Protocol: from human/genomic analysis to chromosomal./genetic diagnosis)" one of "Saibo Kogaku Bessatsu Jikken Purotokooru siriizu (Cell Engineering, 10 Special Edition, Experimental Protocol Series), ed. Ken'ichi Matsubara, Hiroshi Yoshikawa, Shujunsha (Tokyo) and the like. [0208] As used herein, gene expression (e.g., mRNA 15 expression, polypeptide expression) may be "detected" or "quantified" by an appropriate method, including mRNA measurement and immunological measurement. Examples of molecular biological measurement methods include Northern blotting methods, dot blotting methods, PCR methods, and 20 the like. Examples of immunological measurement methods include ELISA methods, RIA methods, fluorescent antibody methods, Western blotting methods, immunohistological staining methods, and the like, where a microtiter plate may be used. Examples of quantification methods include 25 ELISA methods, RIA methods, and the like. A gene analysis method using an array (e.g., a DNA array, a protein array, etc.) may be used. The DNA array is widely reviewed in Saibo-Kogaku [Cell Engineering], special issue, "DNA Microarray and Up-to-date PCR Method", edited by Shujun-sha. 30 The protein array is described in detail in Nat Genet. 2002 Dec; 32 Suppl:526-32. Examples of methods for analyzing gene expression include, but are not limited to, RT-PCR -67- OBKO08 methods, RACE methods, SSCP methods, immunoprecipitation methods, two-hybrid systems, in vitro translation methods, and the like in addition to the above-described techniques. Other analysis methods are described in, for example, 5 "Genome Analysis Experimental Method, Yusuke Nakamura's Lab-Manual, edited by Yusuke Nakamura, Yodo-sha (2002), and the like. All of the above-described publications are herein incorporated by reference. [0209] 10 As used herein, the term "expression level (or amount)" refers to the amount of a polypeptide or mRNA expressed in a subject cell. The term "expression level" includes the level of protein expression of a polypeptide evaluated by any appropriate method using an antibody, 15 including immunological measurement methods (e.g., an ELISA method, an RIA method, a fluorescent antibody method, a Western blotting method, an immunohistological staining method, and the like, or the mRNA level of expression of a polypeptide evaluated by any appropriate method, including 20 molecular biological measurement methods (e.g., a Northern blotting method, a dot blotting method, a PCR method, and the like). The term "change in expression level" indicates that an increase or decrease in the protein or mRNA level of expression of a polypeptide evaluated by an appropriate 25 method including the above-described immunological measurement method or molecular biological measurement method. [02101 As used herein, the terms "transformation", 30 "transduction" and "transfection" are used interchangeably unless otherwise mentioned, and refer to introduction of a nucleic acid into host cells. As a transformation method, -68- OBKO08 any technique for introducing DNA into host cells can be used, including various well-known techniques, such as, for example, the electroporation method, the particle gun method (gene gun), the calcium phosphate method, and the 5 like. [0211] As used herein, the term "transformant" refers to the whole or a part of an organism, such as a cell, which is produced by transformation. Examples of a 10 transformant include prokaryotic cells, yeast, animal cells, plant cells, insect cells and the like. Transformants may be referred to as transformed cells, transformed tissue, transformed hosts, or the like, depending on the subject. As used herein, all of the forms are encompassed, however, 15 a particular form may be specified in a particular context. [0212] Examples of prokaryotic cells include prokaryotic cells of the genera Escherichia, Serratia, Bacillus, Brevibacterium, Corynebacterium, Microbacterium, 20 Pseudomonas, and the like, e.g., Escherichia coli XL1-Blue, Escherichia coli XL2-Blue, Escherichia coli DH1, Escherichia coli MC1000, Escherichia coli KY3276, Escherichia coli W1485, Escherichia coli JM109, Escherichia coli HB101, Escherichia coli No.49, Escherichia coli W3110, 25 Escherichia coli NY49, Escherichia coli BL21(DE3), Escherichia coli BL21(DE3)pLysS, Escherichia coli HMS174(DE3), Escherichia coli HMS174(DE3)pLysS, Serratia ficaria, Serratia fonticola, Serratia liquefaciens, Serratia marcescens, Bacillus subtilis, Bacillus 30 amyloliquefaciens, Brevibacterium ammmoniagenes, Brevibacterium immariophilum ATCC14068, Brevibacterium saccharolyticum ATCC14066, Corynebacterium glutamicum -69- OBKO08 ATCC13032, Corynebacterium glutamicum ATCC14067, Corynebacterium glutamicum ATCC13869, Corynebacterium acetoacidophilum ATCC13870, Microbacterium amnoniaphilum ATCC15354, Pseudomonas sp.D-0110, and the like. 5 [0213] Examples of animal cells include cord blood mononuclear cells, peripheral blood mononuclear cells, Sup Ti cells, and the like. [0214] 10 The term "animal" is used herein in its broadest sense and refers to vertebrates and invertebrates (e.g., arthropods). Examples of animals include, but are not limited to, any of the class Mammalia, the class Aves, the class Reptilia, the class Amphibia, the class Pisces, 15 the class Insecta, the class Vermes, and the like. [0215] As used herein, the term "tissue" in relation to organisms refers to an aggregate of cells having substantially the same function. Therefore, a tissue may 20 be a part of an organ. Organs usually have cells having the same function, and may have coexisting cells having slightly different functions. Therefore, as used herein, tissues may have various kinds of cells as long as a certain property is shared by the cells. 25 [0216] As used herein, the term "organ" refers to a structure which has a single independent form and in which one or more tissues are associated together to perform a specific function. In plants, examples of organs include, 30 but are not limited to, callus, root, stem, trunk, leaf, flower, seed, embryo bud, embryo, fruit, and the like. In animals, examples of organs include, but are not limited -70- OBKO08 to, stomach, liver, intestine, pancreas, lung, airway, nose, heart, artery, vein, lymph node (lymphatic system), thymus, ovary, eye, ear, tongue, skin, and the like. [0217] 5 As used herein, the term "transgenic" refers to incorporation of a specific gene into an organism (e.g., plants or animals (mice, etc.)) or such an organism having an incorporated gene. [02181 10 When organisms of the present invention are animals, the transgenic organisms can be produced by a microinjection method (a trace amount injection method), a viral vector method, an embryonic stem (ES) cell method, a sperm vector method, a chromosome fragment introducing 15 method (transsomic method), an episome method, or the like. These transgenic animal producing techniques are well known in the art. [0219] As used herein, the term "screening" refers to 20 selection of a substance, a host cell, a virus, or the like having a given specific property of interest from a number of candidates using a specific operation/evaluation method. It will be understood that the present invention encompasses viruses having desired activity obtained by 25 screening. [0220] As used herein, the terms "chip" or "microchip" are used interchangeably to refer to a micro-integrated circuit which has versatile functions and constitutes a 30 portion of a system. Examples of a chip include, but are not limited to, DNA chips, protein chips, and the like. [0221] -71 - OBKO08 The herpesvirus promoters of the present invention can be used as an ingredient of a pharmaceutical composition for the treatment, prevention, and/or therapy of lymphatic lineage or hemato-lineage, immune, and 5 infectious diseases. [0222] As used herein, the term "effective amount" in relation to a drug refers to an amount which causes the drug to exhibit intended efficacy. As used herein, an 10 effective amount corresponding to a smallest concentration may be referred to as a minimum effective amount. Such a minimum effective amount is well known in the art. Typically, the minimum effective amount of a drug has been determined or can be determined as appropriate by those 15 skilled in the art. The determination of such an effective amount can be achieved by actual administration, use of an animal model, or the like. The present invention is also useful for the determination of such an effective amount. [02231 20 As used herein, the term "pharmaceutically acceptable carrier" refers to a material which is used for production of a pharmaceutical agent or an agricultural chemical (e.g., an animal drug), and has no adverse effect on effective ingredients. Examples of such a 25 pharmaceutically acceptable carrier include, but are not limited to: antioxidants, preservatives, colorants, flavoring agents, diluents, emulsifiers, suspending agents, solvents, fillers, bulking agents, buffers, delivery vehicles, excipients, and/or agricultural or pharmaceutical 30 adjuvants. [0224] -72- OBKO08 The type and amount of a pharmaceutical agent used in the treatment method of the present invention can be easily determined by those skilled in the art based on information obtained by the method of the present invention 5 (e.g., information relating to a disease) in view of the purpose of use, the target disease (type, severity, etc.), the subject's age, size, sex, and case history, the morphology and type of a site of a subject of administration, or the like. The frequency of subjecting a 10 subject (patient) to the monitoring method of the present invention is also easily determined by those skilled in the art with respect to the purpose of use, the target disease (type, severity, etc.), the subject's age, size, sex, and case history, the progression of the therapy, and the like. 15 Examples of the frequency of monitoring the state of a disease include once per day to once per several months (e.g., once per week to once per month). Preferably, monitoring is performed once per week to once per month with reference to the progression. 20 [0225] As used herein, the term "instructions" refers to a description of the method of the present invention for a person who performs administration, such as a medical doctor, a patient, or the like. Instructions state when to 25 administer a medicament of the present invention, such as immediately after or before radiation therapy (e.g., within 24 hours, etc.). The instructions are prepared in accordance with a format defined by an authority of a country in which the present invention is practiced (e.g., 30 Health, Labor and Welfare Ministry in Japan, Food and Drug Administration (FDA) in the U.S., and the like), explicitly describing that the instructions are approved by the -73- OBKO08 authority. The instructions are so-called package insert and are typically provided in paper media. The instructions are not so limited and may be provided in the form of electronic media (e.g., web sites, electronic mails, 5 and the like provided on the Internet). [0226] In a therapy of the present invention, two or more pharmaceutical agents may be used as required. When two or more pharmaceutical agents are used, these agents 10 may have similar properties or may be derived from similar origins, or alternatively, may have different properties or may be derived from different origins. A method of the present invention can be used to obtain information about the drug resistance level of a method of administering two 15 or more pharmaceutical agents. [0227] Culturing methods used in the present invention are described and supported in, for example, "Doubutsu Baiyosibo Manuaru (Animal Culture Cell Manual), Eeno et al. 20 eds., Kyoritsu shuppan, 1993, the entirety of which is hereby incorporated by reference. [0228] (Methods for producing polypeptides) The polypeptides of the present invention may 25 be produced by culturing a transformant derived from a microorganism or an animal cell possessing a recombinant vector with a DNA encoding the polypeptide of the present invention incorporated therein, in a normal culturing manner, and producing and depositing the polypeptide of the 30 present invention, and recovering the polypeptide of the present invention from the culture of the present invention. [0229] -74- OBK008 The method for culturing the transformant of the present invention in a medium may be conducted according to the normal methods used in the culture of a host. Culture medium for culturing the transformant 5 obtained by using a prokaryotic cell such as E. coli and the like or a eukaryotic cell such as yeast as a host, include those comprising a carbon source, nitrogen source, inorganic salts and the like which can be assimilated by the organism of the present invention, and in which a 10 transformant can efficiently be cultured, which may be natural or synthetic. [0230] As a carbon source, those which can be assimilated by the microorganism can be used and include, for example, glucose, fructose, sucrose, sugar or honey containing the 15 same, starch, starch hydrolysate, organic acids such as acetic acid and propionic acid, alcohols such as ethanol and propanol and the like. [0231] As a nitrogen source, for example, the following can 20 be used: ammonia, a variety of ammonium salts of inorganic or organic acid salt such as ammonium chloride, ammonium sulfate, ammonium acetate, ammonium phosphate, other nitrogen containing substance and the like, peptin, meat extract, yeast extract, corn steep liquid, casein 25 hydrolysate, soybean powder, soybean powder hydrolysate, a variety of fermented bacterial bodies, and the digests thereof and the like. [0232] As inorganic salts, the following can be used for 30 example: potassium primary phosphate, potassium secondary phosphate, magnesium phosphate, magnesium sulfate, sodium chloride, ferrous phosphate, manganese sulfate, copper -75- OBKO08 sulfate, calcium carbonate and the like. Culture will be conducted under aerobic conditions such as shaking or deep aerator agitating culture. [0233] 5 Culture temperature is preferably from 15-40 degrees Celsius. The period of time for culture is usually from five hours to seven days but is not limited thereto. The pH during the culture is kept from 3.0 to 9.0. The adjustment of the pH may be conducted by adding inorganic 10 or organic acid or alkaline solution, urea, calcium carbonate, ammonia and the like. During the culture, antibiotics such as ampicillin or tetracycline or the like may be added as necessary. [0234] 15 When culturing a microorganism which has been transformed using an expression vector containing an inducible promoter, the culture medium may be optionally supplemented with an inducer. For example, when a microorganism, which has been transformed using an 20 expression vector containing a lac promoter, is cultured, isopropyl-$-D-thiogalactopyranoside or the like may be added to the culture medium. When a microorganism, which has been transformed using an expression vector containing a trp promoter, is cultured, indole acrylic acid or the 25 like may be added to the culture medium. A cell or an organ into which a gene has been introduced can be cultured in a large volume using a jar fermenter. Generally used medium for culture are used herein such as Murashige and Skoog (MS) medium, White medium, or these medium 30 supplemented with auxin, cytokine or plant hormones and the like. [0235] -76- OBKO08 For example, when using an animal cell, mediums used for culturing the cell of the subject invention include, for example those generally used such as RMPI1640 medium [The Journal of the American Medical 5 Association,199,519(1967)], Eagle's MEM medium [Science,122,501(1952)] DMEM medium [Virology,8,396(1959)], 199 medium [Proceedings of the Society for the Biological Medicine,73,1(1950)], or such a culture medium supplemented with fetal bovine serum or the like. 10 [0236] Culture is normally carried out for 1 to 7 days under conditions such as pH 6 to 8, 25 to 40 0 C, 5%

CO

2 . An antibiotic, such as kanamycin, penicillin, streptomycin, or the like may be optionally added to the 15 culture medium during cultivation. A polypeptide of the present invention can be isolated or purified from a culture of a transformant, which has been transformed with a nucleic acid sequence encoding the polypeptide, using an ordinary method for 20 isolating or purifying enzymes, which are well known and commonly used in the art. For example, when a polypeptide of the present invention is secreted outside a transformant for producing the polypeptide, the culture is subjected to centrifugation or the like to obtain a soluble fraction. A 25 purified specimen can be obtained from the soluble fraction by a technique, such as solvent extraction, salting out/desalting with ammonium sulfate or the like, precipitation with organic solvent, anion exchange chromatography with a resin (e.g., diethylaminoethyl 30 (DEAE)-Sepharose, DIAION HPA-75 (Mitsubishi Chemical Corporation), etc.), cation exchange chromatography with a resin (e.g., S-Sepharose FF (Pharmacia), etc.), hydrophobic - 77 - OBKO08 chromatography with a resin (e.g., buthylsepharose, phenylsepharose, etc.), gel filtration with a molecular sieve, affinity chromatography, chromatofocusing, electrophoresis (e.g., isoelectric focusing electrophoresis, 5 etc.). [0237] When the polypeptide of the present invention has been expressed and formed insoluble bodies within cells, the cells are harvested, pulverized, and centrifuged. From 10 the resulting precipitate fraction, the polypeptide of the present invention is collected using a commonly used method. The insoluble polypeptide is solubilized using a polypeptide denaturant. The resulting solubilized solution is diluted or dialyzed into a denaturant-free solution or a 15 dilute solution, where the concentration of the polypeptide denaturant is too low to denature the polypeptide. The polypeptide of the present invention is allowed to form a normal three-dimensional structure, and the purified specimen is obtained by isolation and purification as 20 described above. [0238] Purification can be carried out in accordance with a commonly used protein purification method (J. Evan. Sadler et al.: Methods in Enzymology, 83, 458). 25 Alternatively, the polypeptide of the present invention can be fused with other proteins to produce a fusion protein, and the fusion protein can be purified using affinity chromatography using a substance having affinity to the fusion protein (Akio Yamakawa, Experimental Medicine, 13, 30 469-474 (1995)). For example, in accordance with a method described in Lowe et al., Proc. Natl. Acad. Sci., USA, 86, 8227-8231 (1989), Genes Develop., 4, 1288(1990)), a fusion -78- OBKO08 protein of the polypeptide of the present invention with protein A is produced, followed by purification with affinity chromatography using immunoglobulin G. [02391 5 A fusion protein of the polypeptide of the present invention with a FLAG peptide is produced, followed by purification with affinity chromatography using anti FLAG antibodies (Proc. Natl. Acad. Sci., USA, 86, 8227(1989), Genes Develop., 4, 1288 (1990)). 10 The polypeptide of the present invention can be purified with affinity chromatography using antibodies which bind to the polypeptide. The polypeptide of the present invention can be produced using an in vitro transcription/translation system in accordance with a known 15 method (J. Biomolecular NMR, 6, 129-134; Science, 242, 1162-1164; J. Biochem., 110, 166-168 (1991)). [0241] The polypeptide of the present invention can also be produced by a chemical synthesis method, such as 20 the Fmoc method (fluorenylmethyloxycarbonyl method), the tBoc method (t-buthyloxycarbonyl method), or the like, based on the amino acid information thereof. The peptide can be chemically synthesized using a peptide synthesizer (manufactured by Advanced ChemTech, Applied Biosystems, 25 Pharmacia Biotech, Protein Technology Instrument, Synthecell-Vega, PerSeptive, Shimadzu, or the like). [0242] The structure of the purified polypeptide of the present invention can be produced by methods commonly 30 used in protein chemistry (see, for example, Hisashi Hirano. "Protein Structure Analysis for Gene Cloning", published by Tokyo Kagaku Dojin, 1993). The physiological activity of a -79- OBKO08 polypeptide of the present invention can be measured in accordance with a known measurement method. [0243] (Method for producing variant polypeptides) 5 Deletion, substitution or addition of an amino acid of the polypeptide of the present invention may be carried out by site directed mutagenesis, which was well known prior to the present application. Those with one or more amino acids deleted, substituted or added may be prepared 10 in accordance with the methods described in: Molecular Cloning, A Laboratory Manual, Second Edition,Cold Spring Harbor Laboratory Press(1989), Current Protocols in Molecular Biology, Supplement 1-38,JohnWiley & Sons(1987 1997) , Nucleic Acids Research,10,6487(1982) 15 Proc.Natl.Acad.Sci.,USA,79,6409(1982), Gene,34,315(1985) Nucleic Acids Research,13,4431(1985), Proc.Natl.Acad.Sci USA,82,488(1985) , Proc.Natl.Acad.Sci.,USA,81,5662(1984) Science,224,1431(1984) , PCT W085/00817(1985) Nature,316,601(1985) and the like. 20 [0244] (Gene Therapy) In certain embodiments, a nucleic acid comprising a sequence encoding an antibody or a functional derivative thereof is administered for the purpose of gene therapy for 25 treating, inhibiting or preventing a disease or disorder related to abnormal expression and/or activity of a polypeptide used in the present invention. Gene therapy refers to a therapy performed by administering a nucleic acid, which has been expressed or is capable of being 30 expressed, into subjects. In this embodiment of the present invention, a nucleic acid produces a protein -80- OBKO08 encoded thereby and the protein mediates a therapeutic effect. [0245] Any method available in the art for gene 5 therapy may be used in accordance with the present invention. Illustrative methods are described below. [02461 See the following review articles for gene therapy: Goldspiel et al., Clinical Pharmacy 12:488-505 10 (1993); Wu and Wu, Biotherapy 3:87-95 (1991); Tolstoshev, Ann. Rev. Pharmacol. Toxicol. 32:573-596 (1993); Mulligan, Science 260:926-932 (1993); and Morgan and Anderson, Ann. Rev. Biochem. 62:191-217 (1993); and May, TIBTECH 11(5):155-215(1993). Generally known recombinant DNA 15 techniques used for gene therapy are described in Ausubel et al. (eds.), Current Protocols in Molecular Biology, John Wiley & Sons, NY (1993); and Kriegler, Gene Transfer and Expression, A Laboratory Manual, Stockton Press, NY (1990). [0247] 20 (Demonstration of therapeutic activity or preventive activity) The compounds or pharmaceutical compositions of the present invention are preferably tested in vitro, and then in vivo for the desired therapeutic or prophylactic 25 activity, prior to use in humans. For example, in vitro assays to demonstrate the therapeutic or prophylactic utility of a compound or pharmaceutical composition include, the effect of a compound on a cell line or a patient tissue sample. The effect of the compound or composition on the 30 cell line and/or tissue sample can be determined utilizing techniques known to those skilled in the art (including, but not limited to, cell lysis assays). In accordance with -81 - OBKO08 the present invention, in vitro assays which can be used to determine whether administration of a specific compound is indicated, include in vitro cell culture assays in which a patient tissue sample is grown in culture, and exposed to 5 or otherwise administered a compound, and the effect of such compound upon the tissue sample is observed. [0248] (Therapeutic/Prophylactic Administration and Composition) 10 The present invention provides methods of treatment, prevention and prophylaxis by administration to a subject of an effective amount of a component or pharmaceutical composition comprising the promoter of the present invention. In a preferable aspect, the component 15 comprising a promoter may be substantially purified (for example, including the state where the effects are reduced, or a substance causing undesirable side effect is substantially free). Subjects may preferably be an animal including but not limited to: cattle, pigs, horses, 20 chickens, cats, dogs and the like, and preferably primates, and most preferably humans. [0249] When a nucleic acid molecule or polypeptide of the present invention is used as a medicament, the 25 medicament may further comprise a pharmaceutically acceptable carrier. Any pharmaceutically acceptable carrier known in the art may be used in the medicament of the present invention. [0250] 30 Examples of a pharmaceutically acceptable carrier or a suitable formulation material include, but are not limited to, antioxidants, preservatives, colorants, -82- OBKO08 flavoring agents, diluents, emulsifiers, suspending agents, solvents, fillers, bulky agents, buffers, delivery vehicles, and/or pharmaceutical adjuvants. Typically, a medicament of the present invention is administered in the form of a 5 composition comprising a polypeptide or a polynucleotide or a variant or fragment thereof, or a variant or derivative thereof, or an agent capable of modulating any of these substances, with at least one physiologically acceptable carrier, excipient or diluent. For example, an appropriate 10 vehicle may be injection solution, physiological solution, or artificial cerebrospinal fluid, which can be supplemented with other substances which are commonly used for compositions for parenteral delivery. [0251] 15 Acceptable carriers, excipients or stabilizers used herein preferably are nontoxic to recipients and are preferably inert at the dosages and concentrations employed, and preferably include phosphate, citrate, or other organic acids; ascorbic acid, a-tocopherol; low molecular weight 20 polypeptides; proteins (e.g., serum albumin, gelatin, or immunoglobulins); hydrophilic polymers (e.g., polyvinylpyrrolidone); amino acids (e.g., glycine, glutamine, asparagine, arginine or lysine); monosaccharides, disaccharides, and other carbohydrates (glucose, mannose, 25 or dextrins); chelating agents (e.g., EDTA); sugar alcohols (e.g., mannitol or sorbitol); salt-forming counterions (e.g., sodium); and/or nonionic surfactants (e.g., Tween, pluronics or polyethylene glycol (PEG)). [0252] 30 Examples of appropriate carriers include neutral buffered saline or saline mixed with serum albumin. Preferably, the product is formulated as a lyophilizate -83- OBKO08 using appropriate excipients (e.g., sucrose). Other standard carriers, diluents, and excipients may be included as desired. Other exemplary compositions comprise Tris buffer of about pH 7.0-8.5, or acetate buffer of about pH 5 4.0-5.5, which may further include sorbitol or a suitable substitute therefor. [02531 The medicament of the present invention may be administered orally or parenterally. Alternatively, the 10 medicament of the present invention may be administered intravenously or subcutaneously. When systemically administered, the medicament for use in the present invention may be in the form of a pyrogen-free, pharmaceutically acceptable aqueous solution. The 15 preparation of such pharmaceutically acceptable compositions, with due regard to pH,'isotonicity, stability and the like, is within the skill of the art. Administration methods may be herein oral, parenteral administration (e.g., intravenous, intramuscular, 20 subcutaneous, intradermal, to mucosa, intrarectal, vaginal, topical to an affected site, to the skin, etc.). A prescription for such administration may be provided in any formulation form. Such a formulation form includes liquid formulations, injections, sustained preparations, and the 25 like. [0254] The medicament of the present invention may be prepared for storage by mixing a sugar chain composition having the desired degree of purity with optional 30 physiologically acceptable carriers, excipients, or stabilizers (Japanese Pharmacopeia ver. 14, or a supplement thereto or the latest version; Remington's Pharmaceutical -84- OBKO08 Sciences, 18th Edition, A. R. Gennaro, ed., Mack Publishing Company, 1990; and the like), in the form of lyophilized cake or aqueous solutions. [0255] 5 The type and amount of a pharmaceutical agent used in the treatment method of the present invention can be easily determined by those skilled in the art based on information obtained by the method of the present invention (e.g., information relating to a disease) in view of the 10 purpose of use, the target disease (type, severity, etc.), the subject's age, size, sex, and case history, the morphology and type of a site of a subject of administration, or the like. The frequency of subjecting a subject (patient) to the monitoring method of the present 15 invention is also easily determined by those skilled in the art with respect to the purpose of use, the target disease (type, severity, etc.), the subject's age, size, sex, and case history, the progression of the therapy, and the like. Examples of the frequency of monitoring the state of a 20 disease include once per day to once per several months (e.g., once per week to once per month). Preferably, monitoring is performed once per week to once per month with reference to the progression. [0256] 25 (Immune therapy) As used herein the term "vaccine" refers to a composition (for example, suspension or solution) comprising a usually infectious agent or a portion of an infectious agent, an agent (for example, gene sequence) 30 which allows production of such an agent or portion, to induce an active immune response. Antigenic portions constituting vaccines may be a microorganism (such as a -85- OBK008 virus or bacteria or the like), a native product purified from such a microorganism, a synthetic product or genetically engineered proteins, peptides, polysaccharides or similar products and nucleic acid molecules comprising a 5 nucleic acid sequence encoding such proteins. Vaccines express the effects thereof by causing a neutralizing antibody. [0257] As used herein the term "gene vaccine" refers to a 10 composition (for example, suspension or solution or the like) comprising an agent (typically nucleic acid molecule) which is expressed in the subject to be administered and whose expressed product has vaccine action. Typical genetic vaccines may be nucleic acid molecules comprising 15 the nucleic acid sequence encoding a gene product having antigenicity (for example, vectors, plasmids, Naked DNA and the like). [0258] As used herein, immunologic effects of the vaccines 20 according to the present invention can be confirmed by using any method known in the art. Such a method includes, but is not limited to: for example, CTL precursor cell frequency analysis, ELISPOT method, tetramer method, realtime PCR method and the like. As an exemplary 25 description for CTL precursor frequency analysis, peripheral lymphocyte or antigenic peptide and lymphocyte cultured in the presence of IL-2, were subjected to limitation dilution, and IL-2 and feeder cells were cultured under coexistence, and the wells having 30 propagation were stimulated with vaccines or their candidates, and the presence or absence of IFN-y production is measured using ELISA. Herein, positive wells are used -86- OBKO08 to calculate the frequency of CTL precursor cells according to the Poisson Analysis, to evaluate efficacy of the vaccines. As used herein, the number of positive cells is the number of antigen-specific CTLs and the greater the 5 number is, the greater the efficacy of the vaccine. [0259] The present invention may be used as a cancer vaccine. In such a case cancer antigens may be incorporated as a foreign gene. 10 [0260] As used herein, the term "cancer antigen" refers to an antigen molecule which will be newly expressed in association with canceration of a normal cell. Such a cancer antigen includes, but is not limited to, for 15 example: (1) tumor virus derived antigens (for example, T antigens or the like from DNA type tumor virus such as adenovirus, polyoma virus, SV40 and the like). In RNA-type tumor virus of human or mouse, viral envelope proteins are 20 expressed on the cellular surface; (2) tumor specific transplantation antigen (TSTA); this antigen refers to a target antigen of a cancer cell of the same lineage, when the cancer cell is rejected as a result of formation of a specific immune response. Genetic 25 mutations cause variant proteins in a cancer cell, which allows expression thereof on the cellular surface of the cancer cell by association with a molecule of major histocompatibility (MHC) antigen gene complex as peptide fragments, as in other intracellular normal proteins.; 30 (3) tumor associated antigen (TAA): antigens which exhibit specific expression in association with canceration, although it is not necessarily specific to the cancer cell.

-87- OBKO08 For example, it corresponds to a-fetoprotein in liver cancer, carcinoembryonic antigen (CEA) in enteric cancer and the like. These are proteins which are originally present only in normal fetuses, and are not found in the 5 tissues of an adult. However, these proteins are called oncofetal antigens as re-expression will occur with the canceration. [0261] As used herein, any form of cancer antigen may be 10 used, and in particular, a form of carcinoma-related antigen is preferably used. This is because it will be expressed on the surface of a cancer cell upon association with MHC. [0262] 15 As used herein, the term "adjuvant" refers to a substance which increases, or otherwise alters, immune response when mixed with immunogen administered thereinto. Adjuvants are classified in view of minerals, bacteria, plants, synthetic, or products of a host, for example. 20 [0263] As used herein, the term "pathogen" refers to an organism or agent which allows onset of a disease or a disorder to a host. [0264] 25 As used herein, the terms "prophylaxis", "prophylactic" "prevention" and "prevent" refer to a treatment of a disease or a disorder, in which such a disease or disorder should not be caused prior to the actual onset thereof. 30 [0265] As used herein, the terms "therapy", "treatment" and "treat" refer to a treatment in which in -88- OBKO08 the case where such occurs, deterioration of such a disease or disorder is prevented, preferably, at least maintaining the status quo, more preferably, alleviation further more preferably, cleared. 5 [0266] The vaccines of the present invention are preferably tested in vitro, and then in vivo for the desired therapeutic or prophylactic activity, prior to use in humans. For example, in vitro assays to demonstrate the 10 therapeutic or prophylactic utility of vaccines according to the present invention include testing the effect of a vaccine on a cell line or a patient tissue sample. The effect of the vaccines on the cell line and/or tissue sample can be determined utilizing techniques known to 15 those of skill in the art (for example, immunological assay such as ELISA). In vivo tests include but are not limited to: for example, a method for testing whether a neutralizing antibody is raised. [0267] 20 As used herein the term "patient" or "subject" refers to an organism to which the treatment or composition of the present invention is applied. Preferably, the patient may be a human. [02681 25 The present invention provides methods of treatment, inhibition and prophylaxis by administration to a subject of an effective amount of a gene vaccine of the present invention. In a preferred aspect, the compound is substantially purified (e. g., substantially free from 30 substances that limit its effect or produce undesired side effects). [0269] -89- OBKO08 As used herein, the term "administer" means that the polypeptides, polynucleotides or the like of the present invention or pharmaceutical-compositions containing them are incorporated into the cells, tissue or body of an 5 organism either alone or in combination with other therapeutic agents. Combinations may be administered either concomitantly (e.g., as an admixture), separately but simultaneously or concurrently; or sequentially. This includes presentations in which the combined agents are 10 administered together as a therapeutic mixture, and also procedures in which the combined agents are administered separately but simultaneously (e.g., as through separate or the same mucosa into the same individual). "Combination" administration further includes the separate administration 15 of one of the compounds or agents given first, followed by the second. [0270] Administration of vaccines according to the present invention may be conducted in any manner, and preferably it 20 is advantageous to use a needleless syringe. This is because it can administer without causing undue load to a patient. [0271] As used herein the term "needleless syringe" refers 25 to a medical device which transfers a drug solution into the skin by moving a piston by gas pressure or elasticity of an elastic member, thereby administering a drug component into subcutaneous or preferably into the cell's subcutaneous site. 30 [0272] Specifically, for example, Shimajet" (manufactured by Shimadzu, inc.), Medi-Jector Vision" (manufactured by -90- OBK008 Elitemedica), PenJet" m (manufactured by PenJet), which are commercially available. Gene gun (particle gun) refers to a medical and experimental device which allows in vivo gene introduction by accelerating high density particles such as 5 gold or tungsten coated with DNA using gas pressure of helium or the like. Advantageous effects of gene guns include effective intracellular introduction of a low amount of DNA, and stable results have been obtained with different operators. 10 [0273] Specifically, for example, Helios Gene Gun from Bio Rad, USA is commercially available. [0274] As used herein, the term "instructions" refers 15 to a description of the method of the present invention for a person who performs administration, such as a medical doctor, a patient, or the like. Instructions state when to administer a medicament of the present invention, such as immediately after or before radiation therapy (e.g., within 20 24 hours, etc.). The instructions are prepared in accordance with a format defined by an authority of a country in which the present invention is practiced (e.g., Health, Labor and Welfare Ministry in Japan, Food and Drug Administration (FDA) in the U.S., and the like), explicitly 25 describing that the instructions are approved by the authority. The instructions are so-called package insert and are typically provided in paper media. The instructions are not so limited and may be provided in the form of electronic media (e.g., web sites, electronic mails, 30 and the like provided on the Internet). [0275] -91- OBKO08 The judgment of termination of treatment or prevention with a method of the present invention may be supported by the result of an antibody raised using a commercially available assay or device. 5 [0276] The present invention also provides a pharmaceutical package or kit comprising containers loaded with one or more pharmaceutical compositions according to the present invention. A notice in a form defined by a 10 government agency which regulates the production, use or sale of pharmaceutical products or biological products may be arbitrarily attached to such a container, representing the approval of the government agency relating to production, use or sale with respect to administration to 15 humans. [0277] (General techniques used herein) Techniques used herein are within the technical scope of the present invention unless otherwise specified. 20 These techniques are commonly used in the fields of sugar chain science, fluidics, microfabrication, organic chemistry, biochemistry, genetic engineering, molecular biology, microbiology, genetics, and their relevant fields. The techniques are sufficiently well described in documents 25 described below and other documents mentioned herein. [0278] Microfabrication is described in, for example, Campbell, S.A. (1996), The Science and Engineering of Microelectronic Fabrication, Oxford University Press; Zaut, 30 P.V. (1996), Micromicroarray Fabrication: a Practical Guide to Semiconductor Processing, Semiconductor Services; Madou, M.J. (1997), Fundamentals of Microfabrication, CRC1 5 -92 - OBKO08 Press; Rai-Choudhury, P. (1997), Handbook of Microlithography, Micromachining & Microfabrication: Microlithography; and the like, the relevant portions of which are hereby incorporated by reference. 5 [0279] Molecular biology techniques, biochemistry techniques, and microbiology techniques used herein are well known and commonly used in the art, and are described in, for example, Maniatis, T. et al. (1989), Molecular 10 Cloning: A Laboratory Manual, Cold Spring Harbor and its 3rd Ed. (2001); Ausubel, F.M. et al. eds, Current Protocols in Molecular Biology, John Wiley & Sons Inc., NY, 10158 (2000); Innis, M.A. (1990), PCR Protocols: A Guide to Methods and Applications, Academic Press; Innis, M.A. et al. 15 (1995), PCR Strategies, Academic Press; Sninsky, J.J. et al. (1999), PCR Applications: Protocols for Functional Genomics, Academic Press; Gait, M.J. (1985), Oligonucleotide Synthesis: A Practical Approach, IRL Press; Gait, M.J. (1990), Oligonucleotide Synthesis: A Practical Approach, 20 IRL Press; Eckstein, F. (1991), Oligonucleotides and Analogues: A Practical Approac, IRL Press; Adams, R.L. et al. (1992), The Biochemistry of the Nucleic Acids, Chapman & Hall; Shabarova, Z. et al. (1994), Advanced Organic Chemistry of Nucleic Acids, Weinheim; Blackburn, G.M. et al. 25 (1996), Nucleic Acids in Chemistry and Biology, Oxford University Press; Hermanson, G.T. (1996), Bioconjugate Techniques, Academic Press; Method in Enzymology 230, 242, 247, Academic Press, 1994; Special issue, Jikken Igaku (Experimental Medicine) "Idenshi Donyu & Hatsugenkaiseki 30 Jikkenho (Experimental Method for Gene introduction & Expression Analysis)", Yodo-sha, 1997; and the like.

-93- OBKO08 Relevant portions (or possibly the entirety) of each of these publications are herein incorporated by reference. [0280) (Description of preferred embodiments) 5 Hereinafter, the present invention will be described by way of embodiments. Embodiments described below are provided only for illustrative purposes. Accordingly, the scope of the present invention is not limited by the embodiments except as by the appended claims. 10 It will be clearly appreciated by those skilled in the art that variations and modifications can be made without departing from the scope of the present invention with reference to the specification. [02811 15 In an aspect, the present invention provides MIE promoters of HHV (including HHV6A and HHV6B, in particular HHV6B) and HHV7, and/or U95 promoter of HHV7. In particular, it has been discovered that MIE promoter of HHV6B, MIE promoter of HHV7, and U95 promoter of HHV7 are 20 surprisingly enhanced in selectivity to lymphocytes in comparison to IE promoters of HCMV. In particular, adhesive cells (293 cells, Vero cells and the like) only showed one hundredth the activity of that of HCMV IE promoter, whereas in lymphoid cells such as SupTl, U937 and 25 the like, a several fold increase in expression efficiency has been obtained. Such a high level of selectivity or specificity elucidated that it can be applied to the development of a pharmaceutical which is targeted to DNA vaccines, gene therapy, in particular, to lymphocytes. 30 Moreover, in an expression system in vivo, since activities are diminished even in the case of CMV promoters which have potent activity, due to the action of methylase, it is -94- OBK008 understood that the promoter of the present invention may be used to secure expression amount in vivo in blood cells or lymphocyte cells. In genetic diseases, gene therapy of cancer, retroviruses are generally used, however, LTR 5 activity is not so potent, as a promoter, the introduction of the promoter of the present invention upstream of the gene to be expressed allows potent expression in blood cell lineage cells. The present invention is also useful in gene therapy targeting blood cell diseases such as leukemia 10 and the like. Furthermore, RNAi is used as a method of knocking out gene expression, and the promoter of the present invention is used as a promoter for hair-pin type RNA expression vectors, allowing more efficient effects of inhibition of expression in the blood cell lineage. 15 Macrophages or dendritic cells or the like are purified from native peripheral blood using flow cytometry, and these cells are transfected with plasmids constructed so as to express cancer specific antigen or tumor necrosis factor (TNF) or the like under the control of the promoter of the 20 present invention, and reintroduced to the original body after confirmation of expression of cancer antigen, thereby practicing the gene therapy of cancer as a result of efficient activation of tumor antigen specific CTL via Glass I-HLA. 25 [0282] In one embodiment, the promoters of the present invention may have a length of at least 8 contiguous nucleotides. Preferably, the promoter of the present invention includes at least the R3 region or the functional 30 variant thereof, amongst the sequence set forth in SEQ ID NO: 1. More preferably, the promoter of the present invention includes at least the sequence of -574 to -427 -95- OBKO08 from the transcription initiation point of the SEQ ID NO: 1; more preferably, at least the sequence of -1051 to -427 from the transcription initiation point of the SEQ ID NO: 1. This is because it is predicted that these regions have 5 regions having enhancer activity. [0283] In one embodiment, the promoter of the present invention comprises NF-KB and AP-1 motives. [0284] 10 In a preferable embodiment, the promoter of the present invention comprises a sequence set forth in SEQ ID NO: 1, and more preferably consists essentially of the sequence set forth in SEQ ID NO: 1. [0285] 15 In one embodiment, the promoter of the present invention comprises: (a) a polynucleotide having the base sequence set forth in SEQ ID NO: 1, or the base sequence corresponding thereto or a fragment sequence thereof; (b) a polynucleotide of an allelic variant of the base sequence 20 set forth in SEQ ID NO: 1 or the base sequence corresponding thereto or a fragment sequence thereof; (c) a polynucleotide which hybridizes a polynucleotide of any of (a) or (b) and has a biological activity thereof; or (d) a polynucleotide which consists of the base sequence of any 25 of (a) to (c) or a complement sequence thereof with at least 70 % identity, and has a biological activity thereof. As used herein, the biological activity may be promoter and/or enhancer activities but is not limited thereto. Promoter and enhancer activities may be measured using well 30 known technology in the art, and such a technology is described herein and exemplified in the Examples. [0286] -96- OBK008 In one preferred embodiment, the number of substitutions, additions and deletions described in (a) through (d) above may be limited to, for example, preferably 50 or less, 40 or less, 30 or less, 20 or less, 5 15 or less, 10 or less, 9 or less, 8 or less, 7 or less, 6 or less, 5 or less, 4 or less, 3 or less, or 2 or less. The number of substitutions, additions and deletions is preferably small, but may be large as long as the biological activity is maintained (preferably, the activity 10 is similar to or substantially the same as that of HHV6B MIE promoter). [0287] In a preferred embodiment, the identity to any one of the polynucleotides described in (a) to (d) above or 15 a complementary sequence thereof may be at least about 80%, more preferably at least about 90%, even more preferably at least about 98%, and most preferably at least about 99%. [0288] In a preferred embodiment, the nucleic acid 20 molecule of the present invention may have a length of at least 8 contiguous nucleotides. The appropriate nucleotide length of the nucleic acid molecule of the present invention may vary depending on the purpose of use of the present invention. More preferably, the nucleic acid 25 molecule of the present invention may have a length of at least 10 contiguous nucleotides, even more preferably at least 15 contiguous nucleotides, and still even more preferably at least 20 contiguous nucleotides. These lower limits of the nucleotide length may be present between the 30 above-specified numbers (e.g., 9, 11, 12, 13, 14, 16, and the like) or above the above-specified numbers (e.g., 21, 22, ... 30, and the like). The upper limit of the length of -97- OBK008 the polypeptide of the present invention is not limited as long as it can be used for the intended purpose (e.g. promoter). Stringency may be high, or intermediate or low, and the level of stringency may be appropriately determined 5 according to the circumstances. [0289] In a different embodiment, the promoter according to the present invention may have a length of at least 8 contiguous nucleotides. Preferably, the promoter of the 10 present invention includes at least the R2 region or the functional variant thereof, amongst the sequence set forth in SEQ ID NO; 2. More preferably, the promoter of the present invention includes at least the sequence of -388 to +22 from the transcription initiation point of the SEQ ID 15 NO: 2; more preferably, at least the sequence of -493 to +22 from the transcription initiation point of the SEQ ID NO: 2. This is because it is predicted that these regions contain regions having enhancer activity. [0290] 20 In one embodiment, the promoter according to the present invention includes NF-KB motifs (-464 to -478 and 359 to -350 in SEQ ID NO: 2). [0291] In a preferable embodiment, the promoter of the 25 present invention comprises, the sequence set forth in SEQ ID NO: 2, and more preferably, consists essentially of the sequence set forth in SEQ ID NO; 2. [0292] In one embodiment, the promoter of the present 30 invention comprises: (a) a polynucleotide having the base sequence set forth in SEQ ID NO: 2, or the base sequence corresponding thereto or a fragment sequence thereof; (b) a - 98 - OBKO08 polynucleotide of an allelic variant of the base sequence set forth in SEQ ID NO: 2 or the base sequence corresponding thereto or a fragment sequence thereof; (c) a polynucleotide which hybridizes a polynucleotide of any of 5 (a) or (b) and has a biological activity thereof; or (d) a polynucleotide which consists of the base sequence of any of (a) to (c) or a complement sequence thereof with at least 70 % identity, and has a biological activity thereof. As used herein, the biological activity may be promoter 10 and/or enhancer activities but is not limited thereto. Promoter and enhancer activities may be measured using well known technology in the art, and such a technology is described herein and exemplified in the Examples. [0293] 15 In one preferred embodiment, the number of substitutions, additions and deletions described in (a) through (d) above may be limited to, for example, preferably 50 or less, 40 or less, 30 or less, 20 or less, 15 or less, 10 or less, 9 or less, 8 or less, 7 or less, 6 20 or less, 5 or less, 4 or less, 3 or less, or 2 or less. The number of substitutions, additions and deletions is preferably small, but may be large as long as the biological activity is maintained (preferably, the activity is similar to or substantially the same as that of HHV7 MIE 25 promoter). [0294] In a preferred embodiment, the identity to any one of the polynucleotides described in (a) to (d) above or a complementary sequence thereof may be at least about 80%, 30 more preferably at least about 90%, even more preferably at least about 98%, and most preferably at least about 99%. [0295] -99- OBK008 In a preferred embodiment, the nucleic acid molecule of the present invention may have a length of at least 8 contiguous nucleotides. The appropriate nucleotide length of the nucleic acid molecule of the present 5 invention may vary depending on the purpose of use of the present invention. More preferably, the nucleic acid molecule of the present invention may have a length of at least 10 contiguous nucleotides, even more preferably at least 15 contiguous nucleotides, and still even more 10 preferably at least 20 contiguous nucleotides. These lower limits of the nucleotide length may be present between the above-specified numbers (e.g., 9, 11, 12, 13, 14, 16, and the like) or above the above-specified numbers (e.g., 21, 22, ... 30, and the like). The upper limit of the length of 15 the polypeptide of the present invention is not limited as long as it can be used for the intended purpose (e.g. promoter). Stringency may be high, or intermediate or low, and the level of stringency may be appropriately determined according to the circumstances. 20 [0296] In another embodiment, the promoter of the present invention may have a length of at least 8 contiguous nucleotides. Preferably, the promoter of the present invention includes at least the R2 region or the functional 25 variant thereof, amongst the sequence set forth in SEQ ID NO; 12. More preferably, the promoter of the present invention includes at least the sequence of -379 to +16 from the transcription initiation point of the SEQ ID NO: 12; more preferably, at least the sequence of -484 to +16 30 from the transcription initiation point of the SEQ ID NO: 12. This is because it is predicted that these regions containing regions having enhancer activity.

-100- OBKO08 [0297] In one embodiment, the promoter according to the present invention includes NF-KB motifs (-478 to -469 and 373 to -364 in SEQ ID NO: 12). 5 [02981 In a preferable embodiment, the promoter of the present invention comprises, the sequence set forth in SEQ ID NO: 12, and more preferably, consists essentially of the sequence set forth in SEQ ID NO; 12. 10 [0299] In one embodiment, the promoter of the present invention comprises: (a) a polynucleotide having the base sequence set forth in SEQ ID NO: 12, or the base sequence corresponding thereto or a fragment sequence thereof; (b) a 15 polynucleotide of an allelic variant of the base sequence set forth in SEQ ID NO: 12 or the base sequence corresponding thereto or a fragment sequence thereof; (c) a polynucleotide which hybridizes a polynucleotide of any of (a) or (b) and has a biological activity thereof; or (d) a 20 polynucleotide which consists of the base sequence of any of (a) to (c) or a complement sequence thereof with at least 70 % identity, and has a biological activity thereof. As used herein, the biological activity may be promoter and/or enhancer activities but is not limited thereto. 25 Promoter and enhancer activities may be measured using well known technology in the art, and such a technology is described herein and exemplified in the Examples. [0300] In one preferred embodiment, the number of substitutions, additions and deletions described in (a) 30 through (d) above may be limited to, for example, preferably 50 or less, 40 or less, 30 or less, 20 or less, 15 or less, 10 or less, 9 or less, 8 or less, 7 or less, 6 -101- OBK008 or less, 5 or less, 4 or less, 3 or less, or 2 or less. The number of substitutions, additions and deletions is preferably small, but may be large as long as the biological activity is maintained (preferably, the activity 5 is similar to or substantially the same as that of the HHV7 U95 promoter). [0301] In a preferred embodiment, the identity to any one of the polynucleotides described in (a) to (d) above or 10 a complementary sequence thereof may be at least about 80%, more preferably at least about 90%, even more preferably at least about 98%, and most preferably at least about 99%. [0302] In a preferred embodiment, the nucleic acid 15 molecule of the present invention may have a length of at least 8 contiguous nucleotides. The appropriate nucleotide length of the nucleic acid molecule of the present invention may vary depending on the purpose of use of the present invention. More preferably, the nucleic acid 20 molecule of the present invention may have a length of at least 10 contiguous nucleotides, even more preferably at least 15 contiguous nucleotides, and still even more preferably at least 20 contiguous nucleotides. These lower limits of the nucleotide length may be present between the 25 above-specified numbers (e.g., 9, 11, 12, 13, 14, 16, and the like) or above the above-specified numbers (e.g., 21, 22, ... 30, and the like). The upper limit of the length of the polypeptide of the present invention is not limited as long as it can be used for the intended purpose (e.g. 30 promoter). Stringency may be high, or intermediate or low, and the level of stringency may be appropriately determined according to the circumstances.

-102- OBKO08 [03031 In another aspect, the present invention provides a nucleic acid construct comprising a promoter of the present invention (MIE promoter of HHV6, MIE promoter of HHV7, U95 5 promoter of HHV7 and the like). Such a nucleic acid construct has a property of inducing expression in a lymphocyte specific manner, and the utility thereof is high, and exhibits unexpectedly high selectivity in comparison to human cytomegalovirus (HCMV) IE promoter. 10 [0304] Accordingly, in one embodiment, the nucleic acid construct of the present invention comprises a sequence encoding a foreign gene having a different origin than the promoter of the present invention, with a sequence 15 of the present invention operably linked thereto. [0305] Such a foreign gene includes, but is not limited to, for example, those encoding an RNAi molecule, drug resistance, a recessive gene to be deleted, a selective 20 marker and the like. [0306] Preferably, selective markers used in the present invention are those allowing selection in a medium for the host into which the nucleic acid construct is introduced, 25 and for example, these selective markers may be those allowing visible selection in the host into which the nucleic acid construct is introduced, and exemplifies hypoxanthine guanine transferase (hprt) or a fluorescent marker selected from the group consisting of green 30 fluorescent protein (GFP), cyan fluorescent protein (CFP), yellow fluorescent protein (YFP) and red fluorescent protein (dsRed) and the like.

-103- OBKO08 [0307] Preferably, selective markers included in the nucleic acid construct of the present invention are advantageously those substantially exhibiting no toxicity against the host 5 into which the nucleic acid construct is introduced according to the present invention. This is because, when using the present invention for the purpose of therapy or prevention, adverse effects should be preferably none. [0308] 10 Those to be included in the nucleic acid construct according to the present invention include for example, a recessive gene to be deleted. As used herein, a recessive gene to be deleted refers to any recessive gene which exhibits diseased condition when deleted, and 15 includes, but is not limited to, for example: ADA gene (which is related to severe combined immunodeficiency (SCID)), PNP gene (severe combined immunodeficiency (SCID)), y c chain gene (which is related to severe combined immunodeficiency (SCID)), TAP gene (which is related to MHC 20 I deficiency), MHC II gene (which is related to MHC II deficiency), X-linked WASP (which is related to Wiskott Aldrich syndrome), CD40 ligand (which is related to X linked high IgM syndrome), P13K-like gene (which is related to granuloma telangiectaticum) and DNA helicase (which is 25 related to Bloom's syndrome), and the like. [0309] In a preferable embodiment, drugs to be included in the nucleic acid construct of the present invention may be proteineous agents such as a cytokine, a chemokine, a 30 growth factor, a protein hormone, and a peptide hormone such as IFN-a, IFN-y, IL-2, IL-12, G-CSF, GM-CSF and the like.

-104- OBKO08 [0310) In one embodiment, in the nucleic acid construct of the present invention the promoter induces specific expression of the foreign gene in a hemocyto-lineage cell, 5 in particular, in a T cell. [0311] In another aspect, the present invention provides an expression vector comprising the nucleic acid construct according to the present invention. Such an expression 10 vector may include elements essential to expression, which may not exist in the nucleic acid construct of the present invention, for example, terminator, enhancer sequences, in an operably linked manner, which allow expression in the host. 15 [0312] In another preferable embodiment, selective markers may be immortalizing genes (for example bcl-2). Alternatively, selective markers may be hypoxanthine guanine phosphoribosyl transferase (hprt), a gene encoding 20 a toxic product, a toxic gene product depending on a condition in combination with a suicide substrate (for example, herpes simplex virus thymidine kinase (HSV-TK) in combination with acyclovir. [0313] 25 In another aspect, the present invention provides a cell comprising the nucleic acid construct according to the present invention. Such a cell, in the case of a lymphocyte, promotes the expression of a protein encoding a foreign gene. 30 [0314] Preferably, it may be advantageous that the cell of the present invention is heterogenous to the promoter -105- OBKO08 sequence of the present invention. It is one of the surprising effects to have promoter activity even if the cell is heterogenous. A method for introducing a nucleic acid into a cell used in the present invention are well 5 known in the art, and described in detail hereinabove. Alternatively, such a cell may be identified by screening a cell comprising the nucleic acid molecule in a sample comprising the same. The cell comprising the nucleic acid molecule according to the present invention may preferably 10 be in an undifferentiated state. The cells expressing the nucleic acid molecule of the present invention is usually in a state of undifferentiation. Accordingly, a cell into which such a nucleic acid molecule has been introduced so as to be expressed in a controllable manner, may be 15 controlled with respect to the undifferentiated state. Alternatively, such a cell may be used to produce a large amount of the nucleic acid according to the present invention. Such production methods are well known in the art and are described in the literature described herein. 20 [0315] In another aspect, the present invention provides a tissue comprising the nucleic acid construct according to the present invention. Such a nucleic acid sequence is preferably operably linked to a control 25 sequence. Such an organ may be an animal tissue, or a tissue of a different organism such as a plant. Alternatively, such a tissue is used to produce a nucleic acid molecule according to the present invention in a large amount. Such a production method is well known in the art, 30 and described in the reference described herein. [0316] -106- OBKO08 In another aspect, the present invention provides an organ comprising the nucleic acid construct according to the present invention. Such a nucleic acid sequence is preferably operably linked to a control 5 sequence. Such an organ may be an animal organ, or an organ of a different organism such as a plant. Alternatively, such an organ is used to product a nucleic acid molecule according to the present invention in a large amount. Such a production method is well known in the art, 10 and described in the reference described herein. [0317] In another aspect, the present invention provides an organism comprising the nucleic acid construct according to the present invention. Such an organism is 15 used to product a nucleic acid molecule according to the present invention in a large amount. Such a production method is well known in the art, and described in the reference described herein. (0318] 20 In another aspect, the present invention provides a pharmaceutical composition comprising the promoter according to the present invention. As used herein, antigen used may be any proteins desired to raise immune response in a host. Such antigens include, but are 25 not limited to, for example, cancer antigen and the like. Accordingly, the pharmaceutical composition according to the present invention may preferably be DNA vaccine. [0319] In another aspect, the present invention provides a 30 pharmaceutical composition for treating a disease, disorder or condition in which a lymphocyte-specific treatment is desired, which comprises the promoter according to the -107- OBKO08 present invention, and a nucleic acid sequence for the treatment. As used herein, the target of the pharmaceutical composition may appropriately be any diseases, disorders, conditions and the like desired to 5 have lymphocyte specific treatment, and are exemplified by acquired immunodeficiency syndromes. Acquired immunodeficiency syndromes include, severe combined immunodeficiency (SCID), MHC I deficiency, MHC II deficiency, Wiskott-Aldrich syndrome, X-linked high IgM 10 syndrome, granuloma telangiectaticum, Bloom's syndrome and the like. Although not wishing to be bound by theory, acquired immunodeficiency syndrome is caused by some deficiency in a recessive gene (which is herein also called a recessive gene to be deleted). It is thus possible to 15 carry out somatic gene therapy in which this gene to be deleted is introduced to bone marrow cells taken from a patient then the cells are reintroduced into the patient. In this regard, the HHV6B MIE promoter of the present invention is likely employed to increase the gene 20 expression efficiency in a cell differentiated into T cell or macrophage and the like. Introduction of such a gene construct is, for example, possible by using retrovirus and the like. [0320] 25 In a preferable embodiment, the nucleic acid sequences for the treatment include a sequence selected from the group consisting of those encoding cytokines, chemokines, growth factors, protein hormones, peptide hormones, ribozymes and siRNA (HIV-1 gp4l: 30 AATAAGACAGGGCTTGGAAAGACACTTTCCAAGCCCTGTCTTATTTTT(SEQ ID NO: 33)/HIV-1 tat: AAGCATCCAGGAAGTCAGCCTACAAGGCTGACTTCCTGGATGCTTTTT(SEQ ID NO: -108- OBKO08 34)/HTLV-1 tax: GAACATTGGTGAGGAAGGCACAGCCTTCCTCACCAATGTTCTTTTT ( SEQ ID NO: 35)). [0321] 5 In another aspect, the present invention provides a method for expressing a protein in a lymphocyte specific manner, comprising the steps of: A) preparing a nucleic acid construct in which the promoter according to the present invention is operatively linked to a nucleic acid 10 sequence encoding the protein; and B) placing the nucleic acid construct under a condition in which the promoter induces the expression of the nucleic acid sequence encoding the protein. [0322] 15 In another aspect, the present invention provides a kit for expressing a protein in a lymphocyte specific manner, comprising: A) a nucleic acid construct in which the promoter according to the present invention is operatively linked to a nucleic acid sequence encoding the 20 protein; and B) means for placing the nucleic acid construct under a condition in which the promoter induces the expression of the nucleic acid sequence encoding the protein. [03231 25 In another aspect, the present invention further provides a kit for expressing a protein in a lymphocyte specific manner, comprising: A) the promoter according to the present invention; and B) means for producing a nucleic acid construct in which the promoter is linked to a nucleic 30 acid sequence encoding the protein. [0324] -109- OBKO08 In another aspect, the present invention further provides a method for treating or preventing a disease, disorder or condition which requires the expression of a protein in a lymphocyte specific manner, comprising the 5 steps of: A) producing a nucleic acid construct in which the promoter according to the present invention is linked to a nucleic acid sequence encoding the protein; and B) placing the nucleic acid construct under a condition in which the promoter induces the expression of the nucleic 10 acid sequence encoding the protein. [0325] In another aspect, the present invention further provides a kit for treating or preventing a disease, disorder or condition which requires the expression of a 15 protein in a lymphocyte specific manner, comprising: A) a nucleic acid construct in which the promoter according to the present invention is linked to a nucleic acid sequence encoding the protein; and B) means for placing the nucleic acid construct under a condition in which the promoter 20 induces the expression of the nucleic acid sequence encoding the protein. [03261 In another aspect, the present invention further provides a kit for treating or preventing a disease, 25 disorder or condition which requires the expression of a protein in a lymphocyte specific manner, comprising: A) the promoter according to the present invention; and.B) means for producing a nucleic acid construct in which the promoter is linked to a nucleic acid sequence encoding the 30 protein. [0327] -110- OBKO08 In another aspect, the present invention further provides a method for producing a protein, comprising the steps of: A) preparing a nucleic acid construct in which the promoter according to the present invention is linked 5 to a nucleic acid sequence encoding the protein; and B) placing the nucleic acid construct under a condition in which the promoter induces the expression of the nucleic acid sequence encoding the protein. [0328] 10 In another aspect, the present invention further provides a kit for producing a protein, comprising: A) a nucleic acid construct in which the promoter according to the present invention is linked to a nucleic acid sequence encoding the protein; and B) means for placing the nucleic 15 acid construct under a condition in which the promoter induces the expression of the nucleic acid sequence encoding the protein. [0329] In another aspect, the present invention further 20 provides a kit for producing a protein, comprising: A) the promoter according to the present invention; and B) means for producing a nucleic acid construct in which the promoter is linked to a nucleic acid sequence encoding the protein. 25 [0330] In another aspect, the present invention further provides use of the promoter according to the present invention, for manufacture of a pharmaceutical composition for treating or preventing a disease, disorder or condition 30 which requires the expression of a protein in a lymphocyte specific manner. [0331] -111- OBKO08 All scientific literature, patents, published patent applications and publications cited herein are incorporated by reference as if set forth fully herein. [0332] 5 The preferred embodiments of the present invention have been heretofore described for a better understanding of the present invention. Hereinafter, the present invention will be described by way of examples. Examples described below are provided only for illustrative 10 purposes. Accordingly, the scope of the present invention is not limited except as by the appended claims. EXAMPLES [0333] 15 Handling of animals used in the following Examples are in accordance with the provisions set forth in Osaka University. [0334] (EXAMPLE 1: Search for HHV6B promoters and 20 Development of DNA vaccines) With respect to promoters of immediate early protein of HHV-6 (9U,20UMIE,U95,MIE/3KU95/3K, which are different in size), the activity thereof was compared to that of cytomegalovirus (CMV) promoter. With respect to methods, 25 the respective promoter regions were inserted upstream of the luciferase gene of pGL3-Basic Vector (Promega), which were transfected with the respective cells to compare the activity thereof using luciferase activity as reference. Hereinafter, the details of materials and methods are 30 described. [0335] (Materials and Methods) -112 - OBKO08 (Outline) The promoter region of MIE gene of HHV-6B (about 1.2kbp) was cloned, which was linked to an outer membrane glycoprotein of Japan encephalitis virus Beijing-i strain 5 cDNA downstream thereof to construct the plasmid p9u/JEVenv. Green fluorescence protein expression plasmid pEGFP-N1 used was commercially available (available from Clontech). [0336] It was constructed using a plasmid (pcDNA3.1/JEVenv) 10 as reference in which JEVenv was linked downstream of HCMV IE promoter of pcDNA3.lZeo+ vector. Green fluorescence protein expression plasmid pEGFP-N1 used was commercially available (available from BD Biosciences). Furthermore, luciferase expression plasmid used herein was that which 15 has already been constructed (pGL3-Basic; available from Promega). [03371 These plasmids were introduced to the following cells: 293 cell (derived from human kidney), Vero 20 cell(derived from simian kidney), SupT1 cell (derived from human T lymphocyte), U937 cell (derived from human monocyte) and the like (these cells are available from American Type Culture Collection (ATCC), RIKEN Cell Bank, Gene banks and the like). The expression of outer membrane 25 glycoprotein in a cell was studied using indirect fluorescence antibody method using anti-JEV polyclonal antibody, and Western blot with cell extract thereof. [0338] HHV-6MIE promoter region was inserted upstream of 30 firefly luciferase gene of luciferase vector pGL3-Basic (Promega) to form p9u, which was used to prepare truncated -113- OBKO08 mutants by removing bases by Mung Bean Exonuclease from upstream of MIE promoter. [0339] Vero cell was transfected with these truncated 5 mutants and Renilla luciferase expression plasmid for transfection efficiency correction (phRL-SV40) by the lipofection method. Cells were collected 24 hours after the transfection, and cell lysis solution was added thereto. Thereafter, luminescent level was measured in the firefly 10 luciferase and Renilla luciferase in the lysate. In order to correct the efficiency of transfection, the luminescence level of the firefly luciferase was divided by that of Renilla luciferase. [0340] 15 1) Cells The following eight types of cell lines were used for promoter activity measurement. [0341) (1)Vero cell (derived from simian kidney) 20 (2)HEL cell (derived from human embryonic fibroblast cell) (3)L929 cell (derived from murine fibroblast cell) (4)293 cell (derived from human kidney) (5)U373 cell (derived from human glioma) (6)THP-1 cell (derived from human monocyte) 25 (7)SupTl cell (derived from human T cell) (8)U937 cell (derived from human monocyte) (These cells are available from American Type Culture Collection (ATCC)). [0342] 30 2) Plasmids for the measurement of promoter activity In order to measure promoter activity, pGL3-Basic (Promega) having firefly luciferase gene was used. This -114- OBKO08 plasmid has no promoter sequence or enhancer sequence derived from eukaryotic cells, a variety of base sequences are introduced upstream of the luciferase gene, and the amount of luciferase expressed is measured to allow 5 measurement of the promoter activity of the inserted sequence. [0343] 3) Promoter sequence with pGL3-Basic incorporated therein For measurement, as described below, HHV-6MIE 10 promoter region, the promoter region of U95 gene, an immediate early gene of HHV-6 and HCMV MIE promoter region as commercially available expression vectors were used. [0344] HHV-6 promoter region was used after proliferating by PCR 15 and having inserted into pGL3-Basic. [0345] (1) 20u [one with HHV-6MIE promoter region (139381 140624:1243bp) inserted thereinto] (SEQ ID NO: 5) (2) 9u [one with HHV-6MIE promoter region (139381 20 140427:1046bp) inserted thereinto] (SEQ ID NO: 6) (3) MIE [one with HHV-6MIE promoter region (139457 140211:7 54bp) inserted thereinto] (SEQ ID NO: 7) (4) U95 [one with HHV-6 U95 gene promoter region (141823-+ 25 142578:756bp) inserted thereinto] (SEQ ID NO: 8) (5) CMV [one with HCMV MIE promoter excised from commercially available expression vector (pcDNA3.1) inserted thereinto:750bp] (SEQ ID NO: 9) (6) MIE/3K [one with HHV-6MIE promoter region (139443w 30 142578:3136bp) inserted thereinto] (SEQ ID NO: 10) (7) U95/3K [one with HHV-6MIE promoter region (139443-+ 142578:3136bp) inserted thereinto] (SEQ ID NO: 11), as a -115- OBKO08 control, intact pGL3-Basic with no base sequence inserted was used. [0346] Furthermore, a variety of deletion variants were 5 produced. These schematic figures are shown in Figure 5. As variants, the following products were prepared as shown in Figure 5. [0347] (1)9u: -1051 to +1 (SEQ ID NO: 5) 10 (2)9u-d2-7: -814 to +1 (SEQ ID NO: 17) (3)9u-dl-4: -574 to +1 (SEQ ID NO: 18) (4)9u-dl-5: -427 to +1 (SEQ ID NO: 19) (5)9u-dl-7: -350 to +1 (SEQ ID NO: 20) (6)9u-d3-7: -276 to +1 (SEQ ID NO: 21) 15 (7)9u-d5: -240 to +1 (SEQ ID NO: 22) (8)9u-d6: -212 to +1 (SEQ ID NO: 23) (9)9u-d7: -116 to +1 (SEQ ID NO: 24) (10)9u-d8: -77 to +1 (SEQ ID NO: 25) [0348] 20 4) Transfection of a cell with a plasmid Transfection was conducted with Lipofection method using SuperFect (QIAGEN). [0349] In order to correct transfection efficiency, 25 expression plasmids of B-galactosidase (pCH110, Pharmacia) were simultaneously introduced to a cell, and B galactosidase activity was measured. pCH110 expresses B galactosidase under control of the early promoter of SV40. [0350] 30 pGL3construct (8pl) and pCH110 (0.2pl) were mixed together and Superfect reagent (8pl) was added thereto to conduct transfection.

-116- OBKO08 [03511 5) Measurement of luciferase activity Luciferase activity was measured using Luciferase Assay System (Promega). 5 [0352] pGL3construct and pCH110 were cotransfected, and 48 hours later, the cells were recovered. After twice washing with PBS, it was dissolved into 150 fl L of cell lysis solution. One hundred #L of luciferase substrate solution 10 was added to the cell lysis solution supernatant (20 / L), and thirty seconds later, luminescence was measured with a luminometer. [0353] 6) Measurement of B-galactosidase activity 15 B-galactosidase activity was measured using B-gal reporter system (Clontech). To twenty 11 L of cell lysis solution prepared in a similar manner as in the luciferase activity measurement was added 100 P L of luminescent substrate solution, and luminescence was measured after one 20 hour using a luminometer. [0354] 7) Measurement of promoter activity under conditions where cells were activated with TPA The plasmids were transfected with Vero cells and 25 L929 cells, and 24 hours later, the cultures were conducted in the presence and absence of TPA (25ng/ml) for an additional 24 hours. Thereafter, the cells were collected, and measured for the activity of luciferase and B galactosidase. 30 [0355] (Results) 1) Promoter activity of the HHV-6 MIE region: -117- OBK008 Promoter activity of HHV-6 MIE region and promoter activity of HCMV MIE showed different behaviour in endothelial adhesive cells and lymphocyte cells. [0356] 5 (1) Comparison of promoter activities in adhesive cells (Figure 1) The promoter sequence of HHV-6MIE had weaker activity than HCMV in adhesive cells, with some promoter activity. The promoter of U95, a HHV-6 immediate early gene, showed 10 little activity. On the other hand, HCMV MIE promoter showed about 10 to 50 fold more activity than that of HHV-6 MIE promoter in adhesive cells. In particular, in HEL cells and U373 cells, HCMV proliferation competent cells, it showed potent activity. 15 [0357] With respect to the promoter activity of the HHV-6 MIE region, those having the promoter region from 0.7kb to 1.2 kb in length showed substantially the same activity, but reduction in the activity was recognized in the 20 sequence of 3kb. [0358] (2) Comparison of promoter activities in lymphocyte cells (Figure 2) In lymphocyte cells which are proliferation competent 25 cells of HHV-6, the HHV-6 MIE region showed about ten times higher promoter activity than HCMV. In particular, it showed potent activity in THP-1 and U937 which are cell lines of monocytic macrophages. HCMV MIE promoter did not exhibit so strong activity in lymphocytes. 30 [0359] The promoter activity of the HHV-6 MIE region increased the activity thereof in accordance with the -118- OBKO08 length from 0.7 kb to 1.2 kb in the promoter region, however, the length of 3 kb reduced its promoter activity. [0360] 2) Promoter activity of the HHV-6 MIE region when 5 stimulated by a cell with TPA (Figures 3 and 4) Vero cells were stimulated with 12-0-tetradecanoyl phorbol 13-acetate (TPA) to measure the promoter activity of HHV-6 MIE, and all promoter activities were increased, and showed substantially the same level as that of HCMV MIE 10 promoter (Figure 3). [0361] However, in L929 cells, no increase in promoter activity was observed upon cell activation with TPA stimulation (Figure 4). This is believed to be due to the 15 difference in reactivity of TPA on cell type. [0362] In Vero cells, it is believed that TPA increased the HHV-6 MIE promoter activity by inducing a large amount of a variety of transcriptional activation factors. That is, 20 the maximum activity of HHV-6 MIE promoter is as much as HCMV MIE promoter. Therefore, the promoter of the present invention has been demonstrated with respect to its specificity and selectivity. [0363] 25 As such, in the present invention, adhesive cells such as Vero cells, HEL cells, L929 cells, 293 cells, U373 cells, CMV promoters showed ten times more potent activity than that of HHV-6 (Figure 1). However, in cells derived from human lymphocytes such as THP-1 cells, SupT1 cells, 30 U938 cells, several times as much activity as that of CMV promoter was observed in HHV-6 promoter, and it was also -119- OBK008 observed that the more truncated, the more potent activity was found. [0364] Promising promoters from HHV-6 have been confirmed, 5 and from these results, it is understood that these promoters can be applied to DNA vaccines (mumps vaccines) and are extremely promising. [0365] HCMV IE promoter was used as a control to compare and 10 study the HHV-6B MIE promoter activity which has been cloned by the present inventors, in a luciferase expression system. As a result, in adhesive cells such as 293 cells, Vero cells and the like, HHV-6MIE promoter only showed about one tenth as much activity as that of HCMHE promoter. 15 However, in lymphocyte cells such as SupT1, and U937 and the like, it was found that several times greater expression efficiency was obtained. Conducting an assay on the expression of the outer membrane glycoprotein of JEV by using p9u/JEVenv linked to JEV cDNA downstream of the 20 subject promoter, no expression of the JEV protein was detected in any adhesive cells or flowing lymphocytes after 48 hours of transfection. [0366] On the other hand, in pCDNA3.1/JEVenv using the IE 25 promoter of HCMV, the expression of JEV protein was confirmed. [0367] Moreover, in JEV infected Vero cells, which were used as a positive control, outer membrane glycoprotein was 30 readily detected. In order to analyze the cause, transfection efficiency was confirmed using GFP protein expression plasmids. As a result, the introduction -120- OBKO08 efficiency in SupT1 cell was as low as 0.1% or less, however, adhesive 293 cells and Vero cells had a higher introduction efficiency of 45 % and 20 %, respectively. HHV-6 MIE promoter cloned, showed a several times higher 5 expression activity than HCMV MIE promoter in lymphocyte cells. However, expressed gene was not detected with its activity when it was converted to outer membrane glycoprotein of JEV. [0368] 10 It is of interest that the HHV-6 MIE promoter cloned herein showed several times higher expression activity than that of the HCMV-IE promoter in lymphocytes. However, it was unpredictable that when the gene to be expressed had been converted to outer membrane glycoprotein of JEV from 15 the reporter gene, no activity was detected. Therefore, the cause thereof was analyzed as to whether expressed JEV protein acted in a feedback manner, and thus the promoter activity was inhibited in an adverse manner, or that alternatively the expressed antigen is unstable in these 20 cells. [0369] The present Example is summarized as follows: [0370] 1) HHV-6 MIE promoter showed about ten times higher 25 activity than HCMV MIE promoter in lymphocyte cells, in particular, monocyte/macrophage cells. [0371] 2) In epithelial adhesive cells, HHV6 MIE promoter activity was about one tenth of that of HCMV MIE promoter. 30 [0372] 3) HHV-6 MIE promoter is suggested to exhibit substantially the same activity as HCMV MIE promoter under -121- OBK008 conditions where a large amount of a variety of transcriptional factors was induced. [0373] As described above, in the present Example, those 5 which were inserted about 12kbp (6MIEP) upstream of the major immediate early (MIE) gene of HHV-6B and about 700 bp upstream of U95 gene (6U95) upstream of the luciferase gene of pGL3Basic vector (Promega) were used. In comparison to the conventional promoters, in order to study the 10 possibility of the application of these IE promoters to DNA vaccines, comparison with human cytomegalovirus '(HCMV) IE enhancer-promoter (CMVP) in activity were conducted using blood cell lineage cells. In the present Example, immediate early (IE) promoter encoded by human herpes virus 15 6B (HHV-6B) was demonstrated to have extremely high activity in blood cell lineage cells. [0374] 4) Furthermore, as depicted in Figure 7, it was shown that activities in the respective fragments were 20 investigated, and at least -572 to -427 and in particular 1051 to -427 upstream of the initiation point have promoter activity with preferable enhancer activity. The site of 417 to +1 appears to be necessary for promoter activity, and the enhancer activity appears to be necessary to secure 25 specificity. The portions responsible for enhancer activity are elucidated to have NF- K B and AP-1 motifs. Therefore, it appears that it is important to have these motifs in order to have specificity in lymphocytes. [0375] 30 (Example 2: MIE and U95 promoters of HHV-7) Next, experiments relating to promoters from HHV-7 were conducted.

-122- OBK008 [03761 The activity of two immediate early promoters of HHV-7 (7MIEP,7U95P) were compared with the activity of cytomegalovirus (CMV) promoter and HHV-6 IE promoter (9U 5 and U95). Methods of comparison are as follows: the respective promoter regions were inserted upstream of the luciferase gene of pGL3-Basic Vector (Promega), which were transfected with the respective cells to compare the activity thereof using luciferase activity as reference. 10 In order to study the effects of the R2 region present upstream of the respective promoters, a variety of deletion variants have been prepared to measure promoter activity. [0377] (Outline) 15 As a reporter plasmid, about 500 bp from the respective MIE and u95 genes of HHV-7 (7MIEP and 7U95P) were inserted upstream of luciferase gene of pGL3Basic vector (Promega) and used in the present Example. [0378] 20 A reporter plasmid was introduced to T cell lines (Jurkat, Molt-3. SupT-1), and bone marrow cell line (SAS-413) with lipofection methods, and to peripheral blood monocytic cells (PBMC) with electroporation, and luciferase activity was measured. As a result, in comparison with HCMV MIE 25 promoter, HHV-7 MIE promoter and HHV-7 U95 promoter showed several times higher activity than HCMV MIE promoter in T cell lines, and in SAS-413 cells, HCMV MIE promoter has more than ten times higher activity. In the experiment where introduction was made to three lots of PBMC, HHV-7 30 MIE promoter and HHV-7 U95 promoter showed low activity. In comparison with HHV-6 IE promoters (9U and U95), both promoters of HHV-7 showed lower activity in any cell -123- OBK008 species. Further, in the experiments with the deletion mutants of the respective HHV7 MIE promoter and HHV7 U95 promoter, it was shown that although there is some difference from cell type to cell type, R2 is responsible 5 for major enhancer activity against both promoter's activity. In the present Example, it was demonstrated that immediate early (IE) promoter encoded by human herpes virus 7 (HHV-7) has extremely high activity in blood cell lineage cells. 10 [0379] Hereinafter, materials and methods are described in detail. [0380) (Materials and Methods) 15 1) Cells The following five types of cells were used for measuring promoter activity. [0381] (1) Jurkat cell (derived from human T cell) 20 (2) Molt-3 cell (derived from human T cell) (3) SupT1 cell (derived from human T cell) (4) SAS-413 cell (derived from human bone marrow cell) (5) peripheral blood monocytic cells (PBMC) 25 2) plasmids for measuring promoter activity pGL3 Basic (Promega) having Firefly luciferase gene was used for measuring promoter activity. [0382] 3) Promoter sequences inserted into pGL3 Basic 30 HHV-7 MIE gene promoter region (7MIEP) and HHV-7 U95 gene promoter region (U95P) were amplified to about 500bp -124- OBKO08 by PCR, and deletion mutants were prepared for each. These are schematically illustrated in Figure 8. [0383] (1) 7MIEP(-493) [one inserted with upstream 493pb to 5 downstream 22bp from the transcription initiation point of HHV-7 MIE gene] (SEQ ID NO: 26) (2) 7MIEP(-388) [one inserted with upstream 388pb to downstream 22bp from the transcription initiation point of HHV-7 MIE gene] (SEQ ID NO: 27) 10 (3) 7MIEP(-233) [one inserted with upstream 233pb to downstream 22bp from the transcription initiation point of HHV-7 MIE gene] (SEQ ID NO: 28) (4) 7U95P(-484) [one inserted with upstream 484pb to downstream 16bp from the transcription initiation point of 15 HHV-7 U95 gene] (SEQ ID NO: 29) (5) 7U95P(-379) [one inserted with upstream 379pb to downstream 16bp from the transcription initiation point of HHV-7 U95 gene] (SEQ ID NO: 30) (6) 7U95P(-304) [one inserted with upstream 304pb to 20 downstream 16bp from the transcription initiation point of HHV-7 U95 gene] (SEQ ID NO: 31) pGL3 Basic without promoter sequence has been used as a control. [0384] 25 4) Transfection of cell with plasmids Transfection was conducted regarding Jurkat cell, Molt-3 cell, SupT1 cell, and SAS-413 cell with lipofection using Lipofectamine 2000 (Invitrogen), and regarding PBMC, using electroporation with Nucleofector (amaxa). 30 [0385] In order to correct transfection efficiency, expression plasmids of Renilla luciferase (pRL-TK, Promega) -125- OBKO08 were simultaneously introduced to a cell, and Renilla luciferase activity was measured. pRL-TK expresses Renilla luciferase under control of herpes simplex virus thymidine kinase (TK) promoter. 5 [0386] pGL3 reporter (1.2 pg) and pRL-TK (50 ng) were mixed together and 2pl of Lipofectamine 2000 were added thereto to conduct transfection. [0387] 10 5) Measurement of luciferase For the measurement of luciferase activity, Dual Luciferase Reporter Assay System (Promega) was used. [0388] The cells were collected 16 hours after the 15 transfection, and were lysed in cell lysis solution (100pl). To Five pl of supernatant of cell lysis solution, firefly luciferase substrate solution (25pl) was added, and immediately thereafter, luminescence was measured using a luminometer. Next, to the sample after the measurement, 20 Renilla luciferase substrate solution (25pl) was added and immediately thereafter, luminescence was measured using a luminometer. [0389] (Results) 25 1) Activity of promoter region of HHV-7 MIE As a result of experiments using four types of cell lines, when compared with the activity of CMV promoter, 7MIEP(-493) showed about 6-7 times higher activity in Molt 3 cell and SuptTl cell, similar activity in Jurkat cells, 30 and about 1/11 activity in SAS-413 cells. Moreover, when comparing with HHV-6 IE promoters (9U and U95), in all cell types, 7MIEP(-493) showed lower activity (Figure 9).

-126- OBK008 [0390] As a result of experiments using three lots of PBMC, the activity of 7MIEP (-493) was similar or slightly lower than CMV promoter and 9U, and similar or slightly higher 5 than HHV-6 U95 (Figure 10). [0391] 2) Activity of HHV-7 U95 promoter region As a result of experiments using four types of cell lines, when compared with the activity of CMV promoter, 10 7U95P(-484) showed about 2.5 times higher activity in Jurkat cells, four time in Molt-3 cells, twenty times in SupT cells, however, about 1/8 activity in SAS-413 cells. Moreover, when comparing with HHV-6 IE promoters (9U and U95), U95P(-484) showed slightly higher activity in SupT1 15 than U95, however, was about 1/2 of that of 9U, and showed lower activity in other cells (Figure 9). [0392] In an experiment where three lots of PBMC were used, 7U95P(-494) showed only about 1/2 to 1/4 as much promoter 20 activity as that of the others. (Figure 10). [0393] 3) Effects of the R2 region on promoter activity It was elucidated as a result of an experiment where the respective deletion mutants of 7MIEP and 7U95P were 25 introduced into four types of cell lines, that it depends on the type of cell whether the promoter activity is lowered by the deletion of R2. Specifically, 7MIEP showed no effects with the R2 deletion in Jurkat cells, but reduced its activity by about 1/5 to 1/2 in other cell 30 lines. Moreover, 7U95P showed no effects by R2 deletion in SAS-413 cells, but reduced its activity by about 1/7 to 1/2 in other cell lines. (Figure 11).

-127- OBK008 [0394] (Summary) The present Examples are summarized as follows: [0395] 5 1) 7MIEP(-493) and 7U95P(-494) both generally showed more potent activity than CMV promoter in T cell lines, but showed lower activity in the SAS-413 cell, which is a bone marrow cell line. In PBMC, 7MIEPO(-493) showed substantially the same activity as CMV promoter, and 10 7U95P(-494) showed lower activity than CMV promoter. [0396] 2) In comparison with HHV-6 IE promoters, all cell types showed higher activity in two types of IE promoters of HHV-6 (9U and U95) than 7MIEP(-493) and 7U95(-494). 15 [0397] 3) It was shown that the R2 region functions as an enhancer against 7MIEP and 7U95P in a number of cells. Transcriptional factors binding to the R2 region are unidentified, but in view of the fact that the R3 region of 20 HHV-6 functions as an enhancer of the U95 promoter by binding NF-KB, it is highly likely that the NF-KB binding motifs present in a repetitive manner in the R2 region may be responsible for enhancer activity of the R2 region (Figure 8). 25 [0398] (Example 3: Construction of specific deletion system) Knocking out of gene expression in blood cell lineage cells is conducted using an IE promoter and the 30 RNAi method. IE promoters are advantageous for analysis since they are expressed in blood cell lineage cells in a large amount.

-128- OBK008 [0399] 1) Preparation of cells (in the case of macrophages) Healthy human peripheral blood is obtained and separated and purified by density gradient using Ficoll / 5 Hypaque. The PBMCs are cultured in a AIM V serum medium (Life Technologies) supplemented with M-CSF (R&D systems, 100U/ml). The medium is exchanged every three days, and macrophages at Day 6 or 7 are used for experiments. [0400] 10 2) Preparation of siRNA expression retrovirus vector In order to express hair-pin type RNA, a synthetic oligo-DNA comprising "a sense strand target sequence", "a loop sequence", "an antisense strand target sequence" and "a terminator sequence" is prepared. Such a sense strand 15 target sequence, loop sequence, antisense target sequence, terminator sequence may be made using well known technology in the art. Those skilled in the art can readily understand that when actually using these, an appropriate sequence may be employed depending on the actual situation. 20 [0401] The above-mentioned DNA is incorporated into a plasmid vector in which the oligo-DNA is linked downstream of the IE sequence, and of gag, pol and env which are necessary for replication of a retrovirus, and which 25 comprises NeoR gene making use of restriction enzyme sequences and the like. Plasmid vector produced (10pl) is added to 100pl of competent cells and transformation is conducted and cultured for 16 hours at 37 degrees Celsius after plating into LBAmp plate. Colonies obtained by the 30 transformation are cultured on LBApm liquid medium at 37 degrees Celsius for 16 hours, and plasmids are extracted -129- OBKO08 and purified using conventional methods from the culture solution. [0402] Retrovirus packaging cells expressing gag, pol and 5 env are plated on a disc with a 10 cm diameter, and transfection reagent is opened to transfect the plasmid (lOpg). 24-48 hours later, the cells are subjected to limitation dilution into G418 containing medium (500pg/ml) and passaged. 10 [0403] Every three to four days, G418 medium is exchanged and cultured for about two weeks in total. Colonies are collected and at the time where growth is found at a confluent level on a six-well plate, the medium is changed 15 to a G418 free medium and the supernatant is collected 24 hours later. The cells will be stocked. [0404] Retrovirus vectors included in the supernatant are subjected to limitation dilution, and infected into NIH/3T3 20 cells, and colonies grown are counted to calculate the infection value. [0405] 3) Gene introduction experiments using retrovirus vectors 25 Retrovirus vectors are infected with blood cell lineage cells such as macrophages prepared in 1). Immediately after washing, it was plated to form 0.5-2.5 x 104 cells/cm 2 on a plate. Twenty four hours after the infection, the medium is exchanged with G418 containing 30 medium, and every three to four days, medium is exchanged. About two weeks later, gene introduced cells are obtained.

-130- OBKO08 The cells are used to confirm the expression level of the desired knocked out gene. [0406] These experiments are conducted to actually confirm 5 that after gene introduction, lymphocyte specific expression of a foreign gene can be knocked out with the promoter of the present invention. [0407] (Example 4: Specific Expression) 10 Instead of the RNAi of Example 3, a nucleic acid molecule encoding a gene (for example, cytokines such as TGF 8) desired for expression is introduced. [0408] As a result, by conducting similar experiments as in 15 Example 3, after gene introduction, it is confirmed that the promoter according to the present invention actually induces the lymphocyte specific foreign gene expression. [0409] As described above, the present invention is 20 illustrated by way of the preferred embodiments. However, it will be understood that the scope of the present invention should be interpreted only by the accompanying claims. It will also be understood that the patents, patent applications and literature cited herein should be 25 incorporated by reference as if set forth fully herein. Various other modifications will be apparent to and can be readily made by those skilled in the art without departing from the scope and spirit of this invention. Accordingly, it is not intended that the scope of the claims appended 30 hereto be limited to the description as set forth herein, but rather that the claims be broadly construed. [Industrial Applicability) -131- OBKO08 [0410] The present invention provides promoters which selectively induce the expression of protein in an immune responsible cells such as T lymphocytes. The promoters of 5 the present invention are useful in method and medicaments for effectively preventing or treating immune diseases such as acquired immunodeficiency syndromes and the like. The present invention is also useful in the technologies for efficiently conducting gene therapy.

Claims (91)

1. 2. The promoter according to claim 1, which comprises at least eight contiguous nucleotides of the sequence set forth in SEQ ID NO: 1. 10
2. 3. The promoter according to claim 1, which comprises at least the R3 region of the sequence set forth in SEQ ID NO: 1 or a functional variant thereof. 15 4. The promoter according to claim 1, which comprises at least the sequence of -574 to -427 (SEQ ID NO: 13) from the transcription initiation point of the SEQ ID NO: 1.
3. 5. The promoter according to claim 1, which comprises at 20 least the sequence of -1051 to -427 (SEQ ID NO: 14) from the transcription initiation point of the SEQ ID NO: 1.
4. 6. The promoter according to claim 1, which comprises a motif of NF-KB and a motif of AP-1. 25
5. 7. The promoter according to claim 1, which comprises the sequence set forth in SEQ ID NO: 1.
6. 8. The promoter according to claim 1, wherein the promoter 30 comprises: -176- OBKO08 (a) a polynucleotide having the base sequence set forth in SEQ ID NO: 1, or the base sequence corresponding thereto or a fragment sequence thereof; (b) a polynucleotide of an allelic variant of the base 5 sequence set forth in SEQ ID NO: 1 or the base sequence corresponding thereto or a fragment sequence thereof; (c) a polynucleotide which hybridizes a polynucleotide of any of (a) or (b) and has a biological activity thereof; or (d) a polynucleotide which consists of the base sequence 10 of any of (a) to (c) or a complement sequence thereof with at least 70 % identity, and has a biological activity thereof.
7. 9. The promoter according to claim 1, which is at least 10 15 contiguous nucleotides in length.
8. 10. The promoter according to claim 8, wherein the biological activity is the promoter activity. 20 11. A nucleic acid construct comprising the promoter according to claim 1.
9. 12. The nucleic acid construct according to Claim 11, which comprises a sequence encoding a foreign gene, originally 25 not related to the promoter, but now operatively linked to the sequence of the promoter.
10. 13. The nucleic acid construct according to claim 12, wherein the foreign gene encodes an RNAi molecule, a drug, 30 a recessive gene to be deleted, or a selective marker. -177- OBKO08
11. 14. The nucleic acid construct according to claim 13, wherein the selective marker allows selection in a medium of a host in which the nucleic acid construct is introduced. 5 15. The nucleic acid construct according to claim 13, wherein the selective marker allows visual selection in a host in which the nucleic acid construct is introduced.
12. 16. The nucleic acid construct according to claim 13, 10 wherein the selective marker comprises hypoxanthine guanine phosphoribosyl transferase (hprt) or a fluorescent marker selected from the group consisting of green fluorescent protein (GFP), cyan fluorescent protein (CFP), yellow fluorescent protein (YFP) and red fluorescent protein 15 (dsRed).
13. 17. The nucleic acid construct according to claim 13, wherein the selective marker does not substantially exhibit toxicity against the host in which the nucleic acid 20 construct is introduced.
14. 18. The nucleic acid construct according to claim 13, wherein the recessive gene to be deleted is selected from the group consisting of ADA gene, PNP gene, y c chain gene, 25 TAP gene, MHC II gene, X-linked WASP, CD40 ligand, P13K like gene and DNA helicase.
15. 19. The nucleic acid construct according to claim 13, wherein the drug is selected from the group consisting of a 30 cytokine, a chemokine, a growth factor, a protein hormone, and a peptide hormone. -178- OBKO08
16. 20. The nucleic acid construct according to claim 12, wherein the promoter induces specific expression of the foreign gene in a hemocyto-lineage cell, in particular, in a T cell. 5
17. 21. An expression vector comprising the nucleic acid construct according to claim 11.
18. 22. A cell comprising the nucleic acid construct according 10 to claim 11.
19. 23. The cell according to claim 22, wherein the cell is heterogenous to the promoter sequence. 15 24. A tissue comprising the nucleic acid construct according to claim 11.
20. 25. An organ comprising the nucleic acid construct according to claim 11. 20
21. 26. An organism comprising the nucleic acid construct according to claim 11.
22. 27. A pharmaceutical composition comprising the promoter 25 according to claim 1 and a sequence encoding an antigen.
23. 28. The pharmaceutical composition according to claim 27, which is a DNA vaccine. 30 29. A pharmaceutical composition for treating a disease, disorder or condition in which a lymphocyte-specific treatment is desired, which comprises the promoter -179- OBKO08 according to claim 1, and a nucleic acid sequence for the treatment.
24. 30. The pharmaceutical composition according to claim 29, 5 wherein the nucleic acid sequence for the treatment comprises a sequence selected from the group consisting of those encoding cytokines, chemokines, growth factors, protein hormones, peptide hormones, ribozymes and RNAis. 10 31. A method for expressing a protein in a lymphocyte specific manner, comprising the steps of: A) preparing a nucleic acid construct in which the promoter according to claim 1 is operatively linked to a nucleic acid sequence encoding the protein; and 15 B) placing the nucleic acid construct under a condition in which the promoter induces the expression of the nucleic acid sequence encoding the protein.
25. 32. A kit for expressing a protein in a lymphocyte specific 20 manner, comprising: A) a nucleic acid construct in which the promoter according to claim 1 is operatively linked to a nucleic acid sequence encoding the protein; and B) means for placing the nucleic acid construct under 25 a condition in which the promoter induces the expression of the nucleic acid sequence encoding the protein.
26. 33. A kit for expressing a protein in a lymphocyte specific manner, comprising: 30 A) the promoter according to claim 1; and -180- OBKO08 B) means for producing a nucleic acid construct in which the promoter is linked to a nucleic acid sequence encoding the protein. 5 34. A method for treating or preventing a disease, disorder or condition which requires the expression of a protein in a lymphocyte .specific manner, comprising the steps of: A) producing a nucleic acid construct in which the promoter according to claim 1 is linked to a nucleic acid 10 sequence encoding the protein; and B) placing the nucleic acid construct under a condition in which the promoter induces the expression of the nucleic acid sequence encoding the protein. 15 35. A kit for treating or preventing a disease, disorder or condition which requires the expression of a protein in a lymphocyte specific manner, comprising: A) a nucleic acid construct in which the promoter according to claim 1 is linked to a nucleic acid sequence 20 encoding the protein; and B) means for placing the nucleic acid construct under a condition in which the promoter induces the expression of the nucleic acid sequence encoding the protein. 25 36. A kit for treating or preventing a disease, disorder or condition which requires the expression of a protein in a lymphocyte specific manner, comprising: A) the promoter according to claim 1; and B) means for producing a nucleic acid construct in 30 which the promoter is linked to a nucleic acid sequence encoding the protein. -181- OBKO08
27. 37. A method for producing a protein, comprising the steps of: A) preparing a nucleic acid construct in which the promoter according to claim 1 is linked to a nucleic acid 5 sequence encoding the protein; and B) placing the nucleic acid construct under a condition in which the promoter induces the expression of the nucleic acid sequence encoding the protein. 10 38. A kit for producing a protein, comprising: A) a nucleic acid construct in which the promoter according to claim 1 is linked to a nucleic acid sequence encoding the protein; and B) means for placing the nucleic acid construct under 15 a condition in which the promoter induces the expression of the nucleic acid sequence encoding the protein.
28. 39. A kit for producing a protein, comprising: A) the promoter according to claim 1; and 20 B) means for producing a nucleic acid construct in which the promoter is linked to a nucleic acid sequence encoding the protein.
29. 40. Use of the promoter according to claim 1, for 25 manufacture of a pharmaceutical composition for treating or preventing a disease, disorder or condition which requires the expression of a protein in a lymphocyte specific manner.
30. 41. An MIE promoter of HHV7. 30 -182- OBKO08
31. 42. The promoter according to claim 41, which comprises at least eight contiguous nucleotides of the sequence set forth in SEQ ID NO: 2. 5 43. The promoter according to claim 41, which comprises at least the R2 region of the sequence set forth in SEQ ID NO: 2 or a functional variant thereof.
32. 44. The promoter according to claim 41, which comprises at 10 least the sequence of +22 to -233 of the SEQ ID NO: 2.
33. 45. The promoter according to claim 41, which comprises at least the sequence of +22 to -388 of the SEQ ID NO: 2. 15 46. The promoter according to claim 41, which comprises a motif of NF-KB present in the R2 region.
34. 47. The promoter according to claim 41, which comprises the sequence set forth in SEQ ID NO: 15. 20
35. 48. The promoter according to claim 41, wherein the promoter comprises: (a) a polynucleotide having the base sequence set forth in SEQ ID NO. 2, or the base sequence corresponding thereto or 25 a fragment sequence thereof; (b) a polynucleotide of an allelic variant of the base sequence set forth in SEQ ID NO. 2 or the base sequence corresponding thereto or a fragment sequence thereof; (c) a polynucleotide which hybridizes a polynucleotide of 30 any of (a) or (b) and has a biological activity thereof; or -183- OBKO08 (d) a polynucleotide which consists of the base sequence of any of (a) to (c) or a complement sequence thereof with at least 70 % identity, and has a biological activity thereof. 5 49. The promoter according to claim 41, which is at least 10 contiguous nucleotides in length.
36. 50. The promoter according to claim 48, wherein the biological activity is the promoter activity. 10
37. 51. A nucleic acid construct comprising the promoter according to claim 41.
38. 52. The nucleic acid construct according to Claim 51, which 15 comprises a sequence encoding a foreign gene originally not related to the promoter but which is now operatively linked to the sequence of the promoter.
39. 53. The nucleic acid construct according to claim 52, 20 wherein the foreign gene encodes an RNAi molecule, a drug, a recessive gene to be deleted, or a selective marker.
40. 54. The nucleic acid construct according to claim 53, wherein the selective marker allows selection in a medium 25 of a host in which the nucleic acid construct is introduced.
41. 55. The nucleic acid construct according to claim 53, wherein the selective marker allows visual selection in a host in which the nucleic acid construct is introduced. 30
42. 56. The nucleic acid construct according to claim 53, wherein the selective marker comprises hypoxanthine guanine -184- OBKO08 phosphoribosyl transferase (hprt) or a fluorescent marker selected from the group consisting of green fluorescent protein (GFP), cyan fluorescent protein (CFP), yellow fluorescent protein (YFP) and red fluorescent protein 5 (dsRed).
43. 57. The nucleic acid construct according to claim 53, wherein the selective marker does not substantially exhibit toxicity against the host in which the nucleic acid 10 construct is introduced.
44. 58. The nucleic acid construct according to claim 53, wherein the recessive gene to be deleted is selected from the group consisting of ADA gene, PNP gene, y c chain gene, 15 TAP gene, MHC II gene, X-linked WASP, CD40 ligand, P13K like gene and DNA helicase.
45. 59. The nucleic acid construct according to claim 53, wherein the drug is selected from the group consisting of a 20 cytokine, a chemokine, a growth factor, a protein hormone, and a peptide hormone.
46. 60. The nucleic acid construct according to claim 52, wherein the promoter induces specific expression of the 25 foreign gene in a hemocyto-lineage cell, in particular, in a T cell.
47. 61. An expression vector comprising the nucleic acid construct according to claim 51. 30
48. 62. A cell comprising the nucleic acid construct according to claim 51. -185- OBKO08
49. 63. The cell according to claim 62, wherein the cell is heterogenous to the promoter sequence. 5 64. A tissue comprising the nucleic acid construct according to claim 51.
50. 65. An organ comprising the nucleic acid construct according to claim 51. 10
51. 66. An organism comprising the nucleic acid construct according to claim 51.
52. 67. A pharmaceutical composition comprising the promoter 15 according to claim 41 and a sequence encoding an antigen.
53. 68. The pharmaceutical composition according to claim 67, which is a DNA vaccine. 20 69. A pharmaceutical composition for treating a disease, disorder or condition in which a lymphocyte-specific treatment is desired, which comprises the promoter according to claim 41, and a nucleic acid sequence for the treatment. 25
54. 70. The pharmaceutical composition according to claim 69, wherein the nucleic acid sequence for the treatment comprises a sequence selected from the group consisting of those encoding cytokines, chemokines, growth factors, 30 protein hormones, peptide hormones, ribozymes and RNAis. -186- OBKO08
55. 71. A method for expressing a protein in a lymphocyte specific manner, comprising the steps of: A) preparing a nucleic acid construct in which the promoter according to claim 41 is operatively linked to a 5 nucleic acid sequence encoding the protein; and B) placing the nucleic acid construct under a condition in which the promoter induces the expression of the nucleic acid sequence encoding the protein. 10 72. A kit for expressing a protein in a lymphocyte specific manner, comprising: A) a nucleic acid construct in which the promoter according to claim 41 is operatively linked to a nucleic acid sequence encoding the protein; and 15 B) means for placing the nucleic acid construct under a condition in which the promoter induces the expression of the nucleic acid sequence encoding the protein.
56. 73. A kit for expressing a protein in a lymphocyte specific 20 manner, comprising: A) the promoter according to claim 41; and B) means for producing a nucleic acid construct in which the promoter is linked to a nucleic acid sequence encoding the protein. 25
57. 74. A method for treating or preventing a disease, disorder or condition which requires the expression of a protein in a lymphocyte specific manner, comprising the steps of: A) producing a nucleic acid construct in which the 30 promoter according to claim 41 is linked to a nucleic acid sequence encoding the protein; and -187- OBKO08 B) placing the nucleic acid construct under a condition in which the promoter induces the expression of the nucleic acid sequence encoding the protein. 5 75. A kit for treating or preventing a disease, disorder or condition which requires the expression of a protein in a lymphocyte specific manner, comprising: A) a nucleic acid construct in which the promoter according to claim 41 is linked to a nucleic acid sequence 10 encoding the protein; and B) means for placing the nucleic acid construct under a condition in which the promoter induces the expression of the nucleic acid sequence encoding the protein. 15 76. A kit for treating or preventing a disease, disorder or condition which requires the expression of a protein in a lymphocyte specific manner, comprising: A) the promoter according to claim 41; and B) means for producing a nucleic acid construct in 20 which the promoter is linked to a nucleic acid sequence encoding the protein.
58. 77. A method for producing a protein, comprising the steps of: 25 A) preparing a nucleic acid construct in which the promoter according to claim 41 is linked to a nucleic acid sequence encoding the protein; and B) placing the nucleic acid construct under a condition in which the promoter induces the expression of 30 the nucleic acid sequence encoding the protein.
59. 78. A kit for producing a protein, comprising: -188- OBKO08 A) a nucleic acid construct in which the promoter according to claim 41 is linked to a nucleic acid sequence encoding the protein; and B) means for placing the nucleic acid construct under 5 a condition in which the promoter induces the expression of the nucleic acid sequence encoding the protein.
60. 79. A kit for producing a protein, comprising: A) the promoter according to claim 41; and 10 B) means for producing a nucleic acid construct in which the promoter is linked to a nucleic acid sequence encoding the protein.
61. 80. Use of the promoter according to claim 41, for 15 manufacture of a pharmaceutical composition for treating or preventing a disease, disorder or condition which requires the expression of a protein in a lymphocyte specific manner.
62. 81. An U95 promoter of HHV7. 20
63. 82. The promoter according to claim 81, which comprises at least eight contiguous nucleotides of the sequence set forth in SEQ ID NO: 12. 25 83. The promoter according to claim 81, which comprises at least the R2 region of the sequence set forth in SEQ ID NO: 12 or a functional variant thereof.
64. 84. The promoter according to claim 81, which comprises at 30 least the sequence of +16 to -233 of the SEQ ID NO: 12. -189- OBKO08
65. 85. The promoter according to claim 81, which comprises at least the sequence of +16 to -379 of the SEQ ID NO: 12.
66. 86. The promoter according to claim 81, which comprises a 5 motif of NF-KB present in the R2 region.
67. 87. The promoter according to claim 81, which comprises the sequence set forth in SEQ ID NO: 16. 10 88. The promoter according to claim 81, wherein the promoter comprises: (a) a polynucleotide having the base sequence set forth in SEQ ID NO. 12, or the base sequence corresponding thereto or a fragment sequence thereof; 15 (b) a polynucleotide of an allelic variant of the base sequence set forth in SEQ ID NO. 12 or the base sequence corresponding thereto or a fragment sequence thereof; (c) a polynucleotide which hybridizes a polynucleotide of any of (a) or (b) and has a biological activity thereof; or 20 (d) a polynucleotide which consists of the base sequence of any of (a) to (c) or a complement sequence thereof with at least 70 % identity, and has a biological activity thereof.
68. 89. The promoter according to claim 81, which is at least 25 10 contiguous nucleotides in length.
69. 90. The promoter according to claim 88, wherein the biological activity is the promoter activity. 30 91. A nucleic acid construct comprising the promoter according to claim 81. -190- OBKO08
70. 92. The nucleic acid construct according to Claim 91, which comprises a sequence encoding a foreign gene which is not related to the promoter but is operatively linked to the sequence of the promoter. 5
71. 93. The nucleic acid construct according to claim 92, wherein the foreign gene encodes an RNAi molecule, a drug, a recessive gene to be deleted, or a selective marker. 10
72. 94. The nucleic acid construct according to claim 93, wherein the selective marker allows selection in a medium of a host in which the nucleic acid construct is introduced. 15 95. The nucleic acid construct according to claim 93, wherein the selective marker allows visual selection in a host in which the nucleic acid construct is introduced.
73. 96. The nucleic acid construct according to claim 93, 20 wherein the selective marker comprises hypoxanthine guanine phosphoribosyl transferase (hprt) or a fluorescent marker selected from the group consisting of green fluorescent protein (GFP), cyan fluorescent protein (CFP), yellow fluorescent protein (YFP) and red fluorescent protein 25 (dsRed).
74. 97. The nucleic acid construct according to claim 93, wherein the selective marker does not substantially exhibit toxicity against the host in which the nucleic acid 30 construct is introduced. -191- OBK008
75. 98. The nucleic acid construct according to claim 93, wherein the recessive gene to be deleted is selected from the group consisting of ADA gene, PNP gene, y c chain gene, TAP gene, MHC II gene, X-linked WASP, CD40 ligand, P13K 5 like gene and DNA helicase.
76. 99. The nucleic acid construct according to claim 93, wherein the drug is selected from the group consisting of a cytokine, a chemokine, a growth factor, a protein hormone, 10 and a peptide hormone.
77. 100. The nucleic acid construct according to claim 92, wherein the promoter induces specific expression of the foreign gene in a hemocyto-lineage cell, in particular, in 15 a T cell.
78. 101. An expression vector comprising the nucleic acid construct according to claim 91. 20 102. A cell comprising the nucleic acid construct according to claim 91.
79. 103. The cell according to claim 102, wherein the cell is heterogenous to the promoter sequence. 25
80. 104. A tissue comprising the nucleic acid construct according to claim 91.
81. 105. An organ comprising the nucleic acid construct 30 according to claim 91. -192- OBKO08
82. 106. An organism comprising the nucleic acid construct according to claim 91.
83. 107. A pharmaceutical composition comprising the promoter 5 according to claim 81 and a sequence encoding an antigen.
84. 108. The pharmaceutical composition according to claim 107, which is a DNA vaccine. 10 109. A pharmaceutical composition for treating a disease, disorder or condition in which a lymphocyte-specific treatment is desired, which comprises the promoter according to claim 81, and a nucleic acid sequence for the treatment. 15
85. 110. The pharmaceutical composition according to claim 109, wherein the nucleic acid sequence for the treatment comprises a sequence selected from the group consisting of those encoding cytokines, chemokines, growth factors, 20 protein hormones, peptide hormones, ribozymes and RNAis.
86. 111. A method for expressing a protein in a lymphocyte specific manner, comprising the steps of: A) preparing a nucleic acid construct in which the 25 promoter according to claim 81 is operatively linked to a nucleic acid sequence encoding the protein; and B) placing the nucleic acid construct under a condition in which the promoter induces the expression of the nucleic acid sequence encoding the protein. 30
87. 112. A kit for expressing a protein in a lymphocyte specific manner, comprising: -193- OBKO08 A) a nucleic acid construct in which the promoter according to claim 81 is operatively linked to a nucleic acid sequence encoding the protein; and B) means for placing the nucleic acid construct under 5 a condition in which the promoter induces the expression of the nucleic acid sequence encoding the protein.
88. 113. A kit for expressing a protein in a lymphocyte specific manner, comprising: 10 A) the promoter according to claim 81; and B) means for producing a nucleic acid construct in which the promoter is linked to a nucleic acid sequence encoding the protein. 15 114. A method for treating or preventing a disease, disorder or condition which requires the expression of a protein in a lymphocyte specific manner, comprising the steps of: A) producing a nucleic acid construct in which the 20 promoter according to claim 81 is linked to a nucleic acid sequence encoding the protein; and B) placing the nucleic acid construct under a condition in which the promoter induces the expression of the nucleic acid sequence encoding the protein. 25
89. 115. A kit for treating or preventing a disease, disorder or condition which requires the expression of a protein in a lymphocyte specific manner, comprising: A) a nucleic acid construct in which the promoter 30 according to claim 81 is linked to a nucleic acid sequence encoding the protein; and -194- OBKOOB B) means for placing the nucleic acid construct under a condition in which the promoter induces the expression of the nucleic acid sequence encoding the protein. 5 116. A kit for treating or preventing a disease, disorder or condition which requires the expression of a protein in a lymphocyte specific manner, comprising: A) the promoter according to claim 81; and B) means for producing a nucleic acid construct in 10 which the promoter is linked to a nucleic acid sequence encoding the protein.
90. 117. A method for producing a protein, comprising the steps of: 15 A) preparing a nucleic acid construct in which the promoter according to claim 81 is linked to a nucleic acid sequence encoding the protein; and B) placing the nucleic acid construct under a condition in which the promoter induces the expression of 20 the nucleic acid sequence encoding the protein.
91. 118. A kit for producing a protein, comprising: A) a nucleic acid construct in which the promoter according to claim 81 is linked to a nucleic acid sequence 25 encoding the protein; and B) means for placing the nucleic acid construct under a condition in which the promoter induces the expression of the nucleic acid sequence encoding the protein. 30 119. A kit for producing a protein, comprising: A) the promoter according to claim 81; and -195- OBKO08 B) means for producing a nucleic acid construct in which the promoter is linked to a nucleic acid sequence encoding the protein. 5 120. Use of the promoter according to claim 81, for manufacture of a pharmaceutical composition for treating or preventing a disease, disorder or condition which requires the expression of a protein in a lymphocyte specific manner. 10